Impaired K+ Homeostasis and Altered Electrophysiological Properties of Post-Traumatic Hippocampal Glia

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The Journal of Neuroscience, September 15, 1999, 19(18):8152-8162

Impaired K⁺ Homeostasis and Altered Electrophysiological Properties of Post-Traumatic Hippocampal Glia
Raimondo D'Ambrosio, Donald O. Maris, M. Sean Grady, H. Richard Winn, and Damir Janigro
Department of Neurological Surgery, University of Washington, School of Medicine, Harborview Medical Center, Seattle, Washington 98104

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Traumatic brain injury (TBI) can be associated with memory impairment, cognitive deficits, or seizures, all of which can reflectaltered hippocampal function. Whereas previous studies have focusedon the involvement of neuronal loss in post-traumatic hippocampus,there has been relatively little understanding of changes in ionichomeostasis, failure of which can result in neuronal hyperexcitabilityand abnormal synchronization. Because glia play a crucial rolein the homeostasis of the brain microenvironment, we investigatedthe effects of TBI on rat hippocampal glia. Using a fluid percussioninjury (FPI) model and patch-clamp recordings from hippocampalslices, we have found impaired glial physiology 2 d after FPI.Electrophysiologically, we observed reduction in transient outwardand inward K⁺ currents. To assess the functional consequences of these glialchanges, field potentials and extracellular K⁺ activity were recorded in area CA3 during antidromic stimulation.An abnormal extracellular K⁺ accumulation was observed in the post-traumatic hippocampal slices,accompanied by the appearance of CA3 afterdischarges. After pharmacologicalblockade of excitatory synapses and of K⁺ inward currents, uninjured slices showed the same altered K⁺ accumulation in the absence of abnormal neuronal activity. Wesuggest that TBI causes loss of K⁺ conductance in hippocampal glia that results in the failure ofglial K⁺ homeostasis, which in turn promotes abnormal neuronal function.These findings provide a new potential mechanistic link betweentraumatic brain injury and subsequent development of disorderssuch as memory loss, cognitive decline, seizures, andepilepsy.

Key words: glial neuronal interactions; ion homeostasis; patch clamp; potassium selective microelectrodes; epilepsy; traumatic brain injury

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Altered excitability of hippocampal neurons can be responsible for memory impairment, cognitive deficits, and seizures thatare common outcomes of traumatic brain injury (TBI). These neurologicaloutcomes have been well documented, but their pathogenic processesstill remain largely unknown (Annegers et al., 1980; Temkin etal., 1990; Lowenstein et al., 1992; Wheal et al., 1998). Indeed,they can appear in patients who suffered either severe or onlymild forms of TBI (Jennett, 1973; Rimel et al., 1981; Kraus, 1987;Temkin et al., 1996). Thus, the interplay of different pathogenicmechanisms may be involved in post-traumatic altered neuronalexcitability, and consequently in memory and cognitive impairment,seizures, and their progression towardepilepsy.

The majority of the experimental research effort has been thus far focused on neuronal injury in animal models of TBI. Usinglateral fluid percussion injury (FPI), a clinically relevant modelof TBI, Lowenstein et al. (1992) first described the bilateralloss of hilar neurons and its association with dentate gyrus hyperexcitability.This lesion was shown by Smith et al. (1991) to be associatedwith spatial memory impairment. Lyeth et al. (1990) showed thatmidline FPI also causes spatial learning deficits in rats. Survivalof specific neuronal populations and changes in synaptic circuitryor efficacy may all affect the neuronal excitability and synchronization(Schwartzkroin, 1993). Because, ultimately, neuronal firing iscontrolled by ionic gradients, the regulation of the extracellularenvironment and ionic gradients is fundamental for the maintenanceof normal neuronal excitability and function, regardless of noxiouseffects on neurons. Previous work has demonstrated the sensitivityof in situ neurons to elevated extracellular K⁺ and has lead to the acceptance of the "high-K⁺ " model of epileptiform activity (Meltzer, 1899; Feldberg andSherwood, 1957; Zuckermann and Glaser,1968; Traynelis and Dingledine,1988; Jensen et al., 1994). Because potassium homeostasis is regulatedby glia, neuronal excitability may, under certain circumstances,depend on non-neuronalmechanisms.

Glial membrane ion channels participate in the control of ionic homeostasis (Orkand et al., 1966; Newman, 1984; Ballanyi etal., 1987) and, under the condition of pharmacologically impairedK⁺ influx into glia, abnormal accumulation of K⁺ in the extracellular space and increase in neuronal excitabilityoccur (Ballanyi et al., 1987; Janigro et al., 1997; D'Ambrosioet al., 1998b). Given this important role of glia, we were interestedin exploring possible post-traumatic changes in glial membraneproperties and their impact on neuronal excitability. In the presentstudy, we investigated (1) whether TBI causes electrophysiologicalchanges of hippocampal glia, with a special interest in alterationsof potassium conductance that has been observed in other modelsof reactive glia (MacFarlane and Sontheimer, 1997; Bordey andSontheimer, 1998), and (2) whether changes of glial membrane propertiesafter TBI have functional consequences on extracellular K⁺ homeostasis and neuronal excitability. We compared the electrophysiologicalproperties of uninjured and post-traumatic hippocampal glia. AfterFPI, glia demonstrated profound changes in their membrane K⁺ currents, particularly a loss of inward K⁺ current and I_A. These changes were accompanied by impairmentof extracellular K⁺ homeostasis and an associated neuronalhyperexcitability.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fluid percussion injury. Male Sprague Dawley rats (postnatal days 26-31) were anesthetized with 4% halothane, intubated, andmechanically ventilated on 1.5% halothane and 30% O₂. Core temperaturewas maintained at 37°C with a heating pad. The scalp was reflectedto expose the skull, and a 4 mm midline burr hole was drilled2 mm posterior to bregma, with care taken to not penetrate thedura. A female Luer-Lok cannula was then secured to the skullusing a small anchoring screw (inserted into the skull adjacentto the cannula) and methyl-methacrylate cement. The animal wasconnected to the FPI device via the Luer-Lok, and a single 3-4atm pressure pulse was delivered to the closed cranial cavity.The pressure pulse was measured by a transducer (Entran) locatednear the male-female connection. Animals receiving a sham injurywere anesthetized and monitored in an identical manner, but thesingle pressure pulse was generated with the three-way stopcockclosed so that no fluid entered the injury cannula. Animals wereweaned from the ventilator and extubated. During the period ofrecovery from anesthesia and injury, neurological function wasassessed by determining the presence or absence of reflexes, includingpaw-pinch withdrawal, corneal, pinna, respiratory drive, and rightingreflex. Appropriate preinjury and postinjury management was maintainedto insure that all guidelines established by the University ofWashington Animal Care Committee weremet.

GFAP immunoreactivity. At 2 d post-surgery, animals (naïve, sham, and FPI) were anesthetized (pentobarbital overdose) andperfused transcardially with 100 ml of 0.9% saline, followed by200 ml of 4% paraformaldehyde (in 0.1 M phosphate buffer, pH 7.35)over a 30 min period. Brains were removed and post-fixed in theparaformaldehyde solution overnight, then placed in a 30% sucrosein 0.1 M phosphate buffer solution and allowed to sink (24-36hr for cryoprotection). Tissue sectioning (35 µm) was performedon a freezing microtome. For GFAP immunocytochemistry, free-floatingsections were incubated in a solution of 3% normal goat serum(NGS), 0.1% Triton X-100 (TX), and 1.0% bovine serum albumin (BSA)in 0.1 M Tris-buffered saline (TBS; pH 7.4) for 1 hr to blocknonspecific staining. Sections were then transferred to the primaryantisera containing 1:800 dilution of antibody against GFAP (Dako,Carpinteria, CA) in 0.1 M TBS with 3% NGS, 0.1% TX, and 1.0% BSA.After incubation for 24 hr, the tissue was rinsed in 0.1 M TBS,pH 7.4, five times for 10 min. Secondary antibody treatment includeda 1.5 hr incubation in a 1:300 solution of biotinylated goat anti-rabbitIgG in 0.1 M TBS with 3% NGS, 0.1% TX, and 1% BSA. A rinse cyclefollowed, then a 1 hr incubation in a 1:500 Elite avidin-biotinhorseradish peroxidase complex (ABC; Vector Laboratories, Burlingame,CA) in 3% NGS, 0.1% TX, and 1% BSA in 0.1 M TBS. After three rinsesin 0.1 M TBS, and three rinses in 0.1 M TB, pH 7.6, the sectionswere immersed in 7.6 mM nickel ammonium sulfate and 0.05% 3,3-diaminobenzenidine(DAB) in 0.1 M TB solution, pH 7.6, for 5 min, followed by 15min in 0.05% DAB containing 2% D-glucose, 0.04% ammonium-chloride,and 0.0003% glucose oxidase in TB. Four coronal sections of thehippocampus were visually examined per animal, and only the CA3strata radiatum and pyramidale wereconsidered.

We previously observed no difference either in GFAP reactivity or in neuronal excitability between CA1 subregion of naïveand sham-operated rats (D'Ambrosio et al., 1998a). No differencein the morphology or GFAP content of astrocytes was also observedin CA3 of sham-operated and naïve, uninjured animals. Thus, changesin glial electrophysiological properties and in extracellularK⁺ homeostasis are not likely to occur in sham rats. The electrophysiologicalexperiments presented below were obtained by comparison of naïveversus post-FPIhippocampi.

Hippocampal slice preparation. Naïve or 24-48 hr post-FPI rats were anesthetized with halothane and decapitated. Brains wererapidly dissected out in ice-cold, oxygenated modified artificialCSF (aCSF) composed of (in mM): 120 NaCl, 3.1 KCl, 3 MgCl₂, 1CaCl₂, 1.25 KH₂PO₄, 26 NaHCO₃, and 10 dextrose. This low-calciumand high-magnesium solution was used to reduce cellular damagepromoted by Ca²⁺ influx. The two hemispheres were separated by a medial sagittalcut. Each hemisphere was glued to the metal stage of a vibratomeand bathed in the modified aCSF. Slices 400-µm-thick were obtainedcutting perpendicularly to the longitudinal axes of the hippocampi.Slices were then gently transferred with a pipette to a holdingchamber containing aCSF composed of (in mM): 120 NaCl, 3.1 KCl,1 MgCl₂, 2 CaCl₂, 1.25 KH₂PO4, 26 NaHCO₃, and 10 dextrose. Sliceswere allowed to recover at room temperature (24-26°C) for at least1 hr before they were transferred to the recording chamber. Salinesolutions were equilibrated with 95% O₂ and 5% CO₂ to a finalpH of 7.4.

Patch-clamp recordings. Slices were gently transferred to a submersion recording chamber in which they were constantly perfusedwith oxygenated aCSF at a rate of 1-2 ml/min. Complete solutionexchange was achieved within 3 min. All the electrophysiologicalrecordings were performed at room temperature (24-26°C); temperaturefluctuated <1°C during each experiment. Glial cells were selectedfor recordings under visual control with a Nikon microscope equippedwith Hoffman optics at 400× magnification. Patch-clamp recordingswere obtained using an Axopatch 1-C (Axon Instruments, FosterCity, CA) in current- or voltage-clamp mode. Whole-cell pipettesfor ruptured patch were filled with (in mM): 140 K-gluconate,1 MgCl₂, 2 Na₂-ATP, 0.3 NaGTP, 10 HEPES, and 0.5 EGTA, and adjustedto a final pH of 7.2 (with NaOH). The K⁺ reversal potential calculated for our pipette and aCSF solutionwas $-$ 88.7 mV. Pipettes had resistance of 5-6 M $Omega$ . Series resistance(R_S) was compensated at ~80% (lag time, 10 µsec) and monitoredduring the experiment. Recordings were digitized at 48 kHz, filteredat 2-5 kHz, displayed on an oscilloscope, recorded on tape, andacquired on a 486 computer with Clampex 6 (Axon Instruments).Cell membrane capacitance was measured by applying voltage stepsof ±5 mV from the holding potential of $-$ 70 mV and integratingthe capacitive current for the time of the transient. Cell membranepotential was corrected for the tip potential recorded on withdrawalof the micropipette from the cell. Currents reported were notleak-subtracted. The cell input resistance (R_IN) was measuredin voltage clamp. From the holding potential, set to be equalto the resting membrane potential (RMP) (I_holding = 0), voltagesteps of ±5 mV (duration, 100 msec) were applied. The input resistancewas determined from the steady-state current response. Electrophysiologicalexperiments were analyzed with Clampfit (Axon Instruments), anddata were graphed and plotted with Origin 5.0 (MicroCal, Northampton,MA). Specific current densities (picoampere per picofarad) werecalculated by dividing the ionic current by the cell capacitance.Unless otherwise specified, data are expressed as mean ±SEM.

Field recordings. Field potentials were recorded with extracellular pipettes filled with normal aCSF equilibrated with 95%O₂ and 5% CO₂. An Axopatch 1C (Axon Instruments) was used to amplifythe signals. Slice stimulation was carried out using a constantcurrent stimulator (WPI A365; World Precision Instruments). Thestimuli were delivered through a bipolar concentric tungsten electrode.The antidromic stimulation of CA3 pyramidal cells was achievedby placing the electrode in CA2 stratum radiatum to activate Schaffercollaterals. Stimulation rate was set at 0.05, 1, or 3 Hz (400µA; pulse duration, 100 µsec). In a subset of experiments, weblocked neuronal burst discharge by bath-applying the glutamatergicionotrophic receptor antagonist kynurenic acid (1 mM; Sigma, St.Louis, MO). To assess the effect of Cs⁺ (1 mM) on inward K⁺ currents independent from the hyperpolarization-activated mixedcation conductance (I_h), we applied the selective blocker ZD 7288(Zeneca). The experiments with Cs⁺ were performed by adding CsCl (1 mM) to the bathingsolution.

Extracellular potassium measurements by ion-selective microelectrodes. Double-barreled borosilicate capillaries were treatedwith sulfuric acid dissolved in 30% H₂O, washed, and treated withincreasing concentrations of acetone to displace water and improvedrying. Pipettes were dried at 100°C, and were then pulled bya PB-7 vertical puller (Narishige, Tokyo, Japan). Microelectrodeswith tip diameter of ~2 µM were obtained. The ion-sensitive barrelwas treated with trimethylchlorosylane, and its tip was back-filledwith the potassium-selective solution (cocktail "B"; Fluka, Buchs,Switzerland). The rest of the potassium-selective barrel was filledwith 140 mM KCl. The reference barrel was filled with aCSF. AWPI high-impedance dual-differential electrometer (WPI FD223)was used for potassium activity recordings. Signals were amplifiedwith a voltage amplifier (AI2040; Axon Instruments), digitized,and stored on computer. The field potential was subtracted analogicallyfrom the potential recorded from the ion-selective barrel to dissectthe contribution attributable to changes in K⁺ activity. A set of microelectrodes was prepared the day beforethe experiments. Electrodes were calibrated before and after theexperiments to verify their stability over time. We routinelyperformed tests for the selectivity of the electrode when thepotassium channel blocker cesium was used during K⁺-activity recordings. A complete description of the methods usedto compensate for the interfering ion can be found in a varietyof references (Nicolsky, 1937; Eisenman, 1967; Ammann, 1986; Janigroet al., 1997). The relationship between the electromotive forceread by the electrometer and the corresponding [K⁺] was obtained by fitting the Nicolsky-Eisenman equation to theexperimental calibration points. We chose Fluka cocktail "B",a valinomicin-based fluid exchanger, for its selectivity to potassiumin the presence of the interfering ion cesium. We found that 1mM Cs⁺ did not significantly affect the linearity of the response ofour electrodes in the range of extracellular potassium levelsthat we were investigating (from 3 to 7 mM). Each electrode wascalibrated using aCSF in which increasing K⁺ was compensated by removal of isomolar Na⁺. Potassium concentrations of 2, 4.35, 7, 12, and 43.5 mM, withor without CsCl (1 mM), were used for calibration. Only potassium-selectivemicroelectrodes (KSM) showing slopes of 40-60 mV for a 10-foldchange in [K⁺] were used. If, after recording, there was a decrease in responsivenessof the KSM (to a slope of <40 mV/decade), the results were discarded.Maximal care was taken during the experiments to measure the basal[K⁺]_out. To record reliably changes of basal [K⁺]_out, we eliminated DC shifts of potential during KSM insertioninto the slice caused by the interaction of the ion-selectiveexchanger with the lipophylic matter of the tissue (Ammann, 1986);to this end, the electrode tip was twice lowered into an extraneousportion of the hippocampal slice (subiculum or entorhinal cortex).Using this protocol, we observed no further DC shifts during subsequentelectrode insertions into the slice, and thus interpreted theDC shifts as attributable to changes in K⁺ activity (Ammann, 1986; Haglund and Schwartzkroin, 1990). KSMwere consistently at a depth of ~150 µm.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hippocampal CA3 astrocytes are reactive after midline fluid percussion injury

Immunocytochemical studies on the GFAP⁺ cell population of the rat hippocampus were performed to characterize the histologicalnature of astrocytic changes after midline FPI (Fig. 1). We wereparticularly interested in post-traumatic changes of the glialpopulation in CA3 because we previously observed that synchronousneuronal activity arises in this region under the condition ofimpaired glial uptake of K⁺ through membrane ion channels (D'Ambrosio et al., 1998b). Shamsections showed no change in the overall GFAP immunoreactivityin CA3 strata radiatum and pyramidale (Fig. 1C,D). However, profoundchanges were observed in post-FPI sections, where an increasein GFAP immunostaining was evident in both CA3 stratum radiatumand pyramidale (Fig. 1E,F). At higher magnification, post-FPIglia appeared thickened at visual examination because of the increasedGFAP⁺ immunoreactivity (Fig. 1F).

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Figure 1. Reactive response of CA3 astrocytes after midline FPI. GFAP immunoreactivity in slices from control (A, B), sham (C, D), and injured animals (E, F). After midline FPI there is a marked increase in GFAP immunoreactivity of the single cells (100×, A, C, E; 200×, B, D, F). Scale bars, 50 µm.

Passive electrophysiological properties of post-FPI CA3 glia

The electrophysiological changes of post-traumatic glia were studied in acutely isolated hippocampal slices. Glial cells werevisually identified in CA3 strata radiatum and pyramidale as cellswith oval somata of <10 µm diameter. These cells never fired actionpotentials during seal formation (D'Ambrosio et al., 1998b). Identificationof these cells as glia was confirmed by biocytin filling and subsequentmorphological analysis of fixed sections (n = 16). Whole-cellpatch-clamp recordings were obtained from a total of 49 glialcells from naïve or post-traumatic animals. The passive propertiesof control and post-FPI reactive glia are summarized in Table1. With K⁺-gluconate-based intracellular solutions, RMPs spanned a widerange in both normal and post-traumatic glia (from $-$ 77 to $-$ 43mV for control slices, and from $-$ 75 to $-$ 44 mV for post-traumaticslices). No differences were found between RMP distribution incontrol and post-traumatic CA3 glia: recordings obtained fromcontrol CA3 glia yielded an average RMP of $-$ 65.5 ± 2.6 mV (n =28), whereas those obtained from post-FPI slices were $-$ 68 ± 2mV (n = 21; p = 0.2). Mean input resistance (R_IN) computed fromall of the recorded control glial cells was 196 ± 21 M $Omega$ (n = 28),whereas that for post-FPI glia was 163 ± 25 M $Omega$ (n = 21; p = 0.3).


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Table 1. Passive electrophysiological properties of control and post-FPI CA3 glia

Three electrophysiologically distinct types of glia are normally found in the hippocampus. These cells are recognizable bythe expression of distinct whole-cell currents and by their sensitivityto extracellular Cs⁺ (D'Ambrosio et al., 1998b). These three types of glia (complex,inwardly rectifying, and linear cells) could also be found inCA3 of post-FPI slices. However, since the linear type was virtuallyabsent even in control slices (n = 2), we did not consider thesecells for this report. The RMP values for complex and inwardlyrectifying cells did not differ from those of controls. Similarlycontrol and post-FPI complex and inward rectifier cells yieldedsimilar input resistance values (Table 1), and no statisticallysignificant differences were found by comparing across controland injuredgroups.

No changes in membrane capacitance were observed in inwardly rectifying glia 24-48 hr after midline FPI. Conversely, a significantdecrease in cell membrane capacitance was found in complex cells(Table 1). Control complex cells had a capacitance of 34 ± 5pF (n = 10) whereas complex cells in post-FPI slices had 15 ±7 pF (n = 10; p = 0.004). Biocytin filling and postelectrophysiologicalanalysis of the fixed section revealed that all the recoveredcomplex cells had oligodendrocyte-like morphology (n = 8 cells;Fig. 2), whereas all the recovered inwardly rectifying cells showedastrocytic morphology (n = 4 cells). Cell-to-cell coupling amongcomplex cells was never observed. Thus, the decrease in membranecapacitance could not be accounted for by changes in cell-to-cellcoupling.

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Figure 2. Post-FPI CA3 complex cells have oligodendrocyte-like morphology. Photomicrograph (A) and camera lucida drawings (B-D; C, same cell as in A) of biocytin-filled complex cells located in CA3 stratum radiatum. All the complex cells recovered for morphological analysis showed oligodendrocyte-like morphology (n = 8). These cells are characterized by fine long processes that show periodic swellings and that radiate from small somata. Scale bar, 50 µm.

Complex and inward rectifier glia lose inward potassium current after fluid percussion injury

Complex and inward rectifier glial cells are endowed with inward K⁺ currents that may be involved in buffering of extracellular K⁺ (Newman, 1984, 1995; Janigro et al., 1997; McKhann et al., 1997;D'Ambrosio et al., 1998b). Inward K⁺ current expressed in glia are sensitive to blockade by extracellularCs⁺ (Ransom and Sontheimer, 1995; Janigro et al., 1997; D'Ambrosioet al., 1998b). We used bath application of this blocker duringwhole-cell glial recordings to measure the inward K⁺ current in control and FPI tissue. For both complex and inwardrectifier glial cells, we found a significant loss of inwardlyrectifying K⁺ currents after FPI. To quantify the expression of inward rectifierpotassium currents in control and post-FPI slices, we used thesame voltage command protocol previously employed to characterizethese cell types (D'Ambrosio et al., 1998b). Voltage commandsconsisted of 750 msec duration ramps, from $-$ 170 to +100 mV (froma holding potential of $-$ 70 mV). Under these voltage command conditions,complex and inwardly rectifying glial cells normally showed Cs⁺-sensitive inwardly rectifying K⁺ currents. Bath application of Cs⁺ (1 mM) yielded a different degree of blockade depending on thecell type and the experimental condition (control vs FPI). Foreach cell, we computed the percentage of Cs⁺-sensitive current (I_Cs) present at any given membrane potentialwith respect to the total whole-cell current at that potential(I_max). This ratio is an indicator not only of the cell type endowedwith inward potassium current (i.e., complex vs inward rectifiercells) but also of the effect of FPI. Figure 3 shows voltage-clamprecording and the pharmacological isolation of the inward currentin complex cells from control and post-FPI hippocampal slices.Complex cells in normal hippocampal slices exhibited large inwardCs⁺-sensitive current components, particularly at hyperpolarizedlevels (I_Cs/I_max= 81 ± 11% at $-$ 140 mV; n = 7). In contrast, complexcells in post-FPI hippocampal slices displayed little Cs⁺ sensitivity i.e., exhibited only a small Cs⁺-sensitive component of the whole-cell inward currents (I_Cs/I_max=28 ± 8% at $-$ 140 mV; n = 7). The inward current components thatwere Cs⁺-insensitive were small in control complex cells [(I_max $-$ I_Cs)/I_max=19 ± 11% at $-$ 140 mV; n = 7). Conversely, post-FPI complex cellsdisplayed large Cs⁺-insensitive current component [(I_max $-$ I_Cs)/I_max = 72 ± 8% at $-$ 140 mV; n = 7). We performed the same type of analysis from atotal of 23 inward rectifier glial cells (Fig. 4). Inward rectifierglia in normal hippocampal slices exhibited proportionally moreCs⁺-sensitive inward current than those found in post-FPI hippocampalslices. Bath application of Cs⁺ (1 mM) revealed that inward rectifier cells in normal hippocampuswere characterized by an I_Cs/I_max of 16 ± 1% (at $-$ 140 mV; n =13). In contrast, inward rectifier cells from post-FPI hippocampusexhibited an I_Cs/I_max of 8 ± 2% (at $-$ 140 mV; n = 10). The inwardcurrent component that was Cs⁺-insensitive in control inward rectifier cells was 84 ± 1% (at $-$ 140 mV; n = 13) and 92 ± 2% in post-FPI inward rectifier cells(at $-$ 140 mV; n = 10).

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Figure 3. Complex glial cells lose inward K⁺ currents after midline FPI. Complex cells in control hippocampal slices exhibited large Cs⁺-sensitive currents (A, top and bottom panels) and were characterized by a large Cs⁺-sensitive component (81 ± 11% at $-$ 140 mV; n = 7). In contrast, complex cells in post-FPI hippocampal slices displayed little Cs⁺-sensitivity (B, top and bottom panels) and showed a decreased Cs⁺-sensitive component of the whole-cell inward currents (28 ± 8% at $-$ 140 mV; n = 7). C, The percentage of Cs⁺-sensitive currents (I_Cs) for complex cells in normal and post-FPI hippocampus is shown for membrane potentials from $-$ 140 to $-$ 80 mV. Voltage commands consisted of ramps from $-$ 170 to +100 mV over 750 msec from holding potential of $-$ 70 mV.

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Figure 4. Inward rectifier glial cells lose inward K⁺ currents after midline FPI. Inward rectifier glia in normal hippocampal slices exhibited Cs⁺-sensitive currents (A, top and bottom panels) that were higher than those found in inward rectifier cells in post-FPI hippocampal slices (B, top and bottom panels). C, The percentage of Cs⁺-sensitive currents for inward rectifier cells in normal and post-FPI hippocampus is shown for membrane potentials from $-$ 140 to $-$ 80 mV. Bath application of Cs⁺ 1 mM revealed that inward rectifier cells in normal hippocampus were characterized by 16 ± 1% Cs⁺-sensitive current (at $-$ 140 mV; n = 13). In contrast, inward rectifier cells in post-FPI hippocampus showed decreased Cs⁺-sensitivity of the inward currents to 8 ± 2% (at $-$ 140 mV; n = 10). Voltage commands consisted of ramps from $-$ 170 to +100 mV over 750 msec from holding potential of $-$ 70 mV.

The discrepancy between loss of Cs⁺-sensitive K⁺ currents and no change in R_IN may be accounted for by inward rectifier channelsbeing located in fine distal processes of the glial membrane andthus undetectable by small voltage commands used to test R_IN aroundcell RMP. We thus measured the absolute inward current evokedby the ramp command at $-$ 140 mV, a voltage command sufficient tocause potential changes even in distal processes. For this measurementwe used only cells that appeared to be isolated, as determinedby their membrane capacitance and by biocytin filling (D'Ambrosioet al., 1998b). Complex cells in normal hippocampal slices exhibiteda mean inward current of $-$ 350 ± 33 pA (at $-$ 140 mV; n = 10). Incontrast, complex cells in post-FPI slices exhibited significantlyless inward current ( $-$ 210 ± 43 pA at $-$ 140 mV; n = 10; p = 0.02).We performed the same type of analysis from isolated inward rectifierglial cells. In normal hippocampal slices, isolated inward rectifiercells had an inward current of $-$ 1130 ± 160 pA (at $-$ 140 mV; n =12). In contrast, isolated inward rectifier cells in post-FPIslices had an inward current of only $-$ 620 ± 110 pA (at $-$ 140 mV;n = 10; p = 0.02). Thus, an increase in membrane resistance inducedby FPI was detectable at hyperpolarizedpotentials.

Complex cells lose transient outward K⁺ current after fluid percussion injury

CA3 complex cells are endowed with transient outward potassium currents evoked by membrane depolarization (D'Ambrosio et al.,1998b). Owing to its activation properties, this current transientlyactivates at membrane potentials positive to $-$ 40 mV (Bordey andSontheimer, 1997). Thus, this current may have a role in couplingglial cell membrane potential to pronounced changes in extracellularK⁺. We compared the density of this current in complex cells incontrol and post-FPICA3.

Whole-cell recordings performed from complex cells revealed that the transient outward current is dramatically reduced afterFPI (Fig. 5). Complex cells were voltage-clamped at a holdingpotential of $-$ 70 mV. A conditioning voltage step to $-$ 80 mV (80msec) was applied to deinactivate the transient current. Whendepolarizing voltage steps were applied (in 10 mV increments),a transient outward current that resembled the "A-type" current(I_A) was activated in glia from normal slices (Fig. 5A). Whenthe conditioning step was set to $-$ 40 mV, the transient outwardcurrent was inactivated completely, and only a sustained currentwas observed (Fig. 5B). Separation of the inactivating currentwas obtained as difference of whole-cell currents evoked by thedeinactivating and inactivating protocols (Fig. 5C). Complex cellsin CA3 of control rats showed high density of transient outwardcurrent (30 ± 10 pA/pF at 100 mV; Fig. 5G, filled circles). Incontrast, post-FPI complex cells showed a dramatic loss of thetransient outward current (2 ± 1 pA/pF at 100 mV; p < 0.02; Fig.5G, open circles). No transient outward current was detectablewith the activation protocol (Fig. 5D) or as the difference ofthe whole-cell currents evoked in presence and in absence of thedeactivating conditioning step (Fig. 5C).

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Figure 5. Complex glial cells lose K⁺ transient outward currents after midline FPI. Complex cells are endowed with depolarization-induced transient outward currents that can be induced by voltage commands consisting of a conditioning step to $-$ 80 mV (holding potential, $-$ 70 mV) followed by depolarization in 10 mV increments (A). When the conditioning step was to $-$ 40 mV, the transient outward current was inactivated, and only a delayed rectifier current was observed (B). C, Current computed as difference between protocol A and B. The dashed line represents the time where the current is measured and plotted in G. Post-FPI complex cells showed a dramatic loss of the transient outward current (D, E), and no current is detectable as difference (F). G, Relationship between the peak evoked current density (dashed line) in normal and post-FPI complex cells at membrane potentials from $-$ 80 to +100 mV. The extrapolated reversal potential was $-$ 89.7 mV, which is near the predicted reversal potential for K⁺ currents ( $-$ 88.7 mV). Asterisks represent statistical significance at p < 0.02.

Basal extracellular K⁺ is elevated in post-FPI slices

The data thus far show that expression of inward and transient outward K⁺ currents are decreased at early time points after FPI. To assesspotential functional effects of decreasing glial K⁺ currents after trauma, we focused on activity in the CA3 subfield.This region of the hippocampus was found to be predominantly endowedwith complex and inward rectifier cells (D'Ambrosio et al., 1998b).We first measured the K⁺-activity in CA3 strata radiatum and pyramidale (Fig. 6). TheKSM was positioned just above the tissue, and the electrometerwas set to a reference potential reflecting the level of K⁺ in the bath. The electrode was then gently inserted into thetissue at a depth of ~150 µm, and after 1 min, it was repositionedinto the bathing solution above the slice. For every slice, thesubregions CA3a, CA3b, and CA3c were tested. In control slices,little or no changes in the reading of the electrometer were observed(Fig. 6A). When the same procedure was performed in post-FPI slices,positive DC shifts of the potential were detected, suggestingincreased basal K⁺ activity (Fig. 6B). The DC shifts in the potential recorded were $-$ 0.08 ± 0.06 mV in control (n = 12), and 2.06 ± 0.2 mV in post-FPIslices (n = 9; p < 0.01; Fig. 6C). The corresponding basal [K⁺]_out was 4.34 ± 0.01 mM in control slices, and 4.78 ± 0.05 mMin post-FPI slices (Fig. 6D). No differences in basal [K⁺]_out were found within CA3 subregions in the same slice.

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Figure 6. CA3 basal [K⁺]_out is elevated after midline FPI. K⁺ activity recording in CA3 strata radiatum and pyramidale. The KSM was positioned just above the tissue, and the potential read was zeroed. The electrode was then gently inserted at a depth of ~150 µm. A, In control slices, we observed either little or no DC shifts of the potential corresponding to little or no changes of potassium activity in the extracellular space of the slices. Top and bottom panels correspond to two experiments from two different slices. B, In post-FPI slices, the insertion of the electrode always elicited positive DC shifts, corresponding to increase of K⁺ activity. Top and bottom panels correspond to two experiments from two different post-FPI slices. C, The DC shifts in potential recorded were $-$ 0.08 ± 0.06 mV in control (n = 12) and 2.06 ± 0.2 mV in post-FPI slices (n = 9; p < 0.01). D, The corresponding basal [K⁺]_out was 4.34 ± 0.01 mM in control slices and 4.78 ± 0.05 mM in post-FPI slices. Black and white bars represent duration of electrode insertion and extraction, respectively.

Accumulation of extracellular K⁺ during neuronal activity is abnormal in post-FPI slices

To examine the dynamics of extracellular K⁺ accumulation in control and post-FPI slices, field potentials and extracellularK⁺ activity were recorded during neuronal stimulation. Schaffercollaterals (SC) were stimulated for 4 min at 1 Hz to antidromicallyactivate CA3 pyramidal cells. A low impedance field electrodeand a KSM were placed in CA3 stratum radiatum to record activityin response of stimulation (Fig. 7).

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Figure 7. Neuronal stimulation induces abnormal accumulation of extracellular K⁺ and burst discharge in post-FPI slices. Field electrode and KSM were placed in CA3 stratum radiatum. Stimulating electrode was placed in CA2 stratum radiatum. K⁺ activity recordings were performed during 0.05 and 1 Hz antidromic stimulation. A, Control slices (filled circles) had a basal [K⁺]_out similar to that of bathing aCSF. Antidromic stimulation at 1 Hz for 4 min induced a transient elevation of [K⁺]_out to ~5 mM and its recovery toward baseline values within the fourth minute. During the following 0.05 Hz, [K⁺]_out transiently decreased to ~4 mM and then recovered. Post-FPI slices (empty circles) had elevated basal [K⁺]_out during stimulation at 0.05 Hz. When the high-frequency stimulation was performed [K⁺]_out transiently increased to 5.4 mM and then decreased to 5 ± 0.05 mM without reaching the baseline value (asterisk; p < 0.001). During the following 0.05 Hz, [K⁺]_out transiently decreased to ~4.7 mM. B, Post-FPI CA3 develops frequency-dependent afterdischarges for antidromic stimulation. In control, only a small fraction of slices developed afterdischarges during antidromic 1 Hz stimulation (28%; 2 of 7 slices). Post-FPI slices showed a higher excitability. They did not show afterdischarges during 0.05 Hz stimulation, but afterdischarges appeared during 1 Hz stimulation (80%; 8 of 10 slices). Two traces obtained at the end of a minute of 1 Hz-stimulation are showed overlapped.

Control slices (Fig. 7, filled circles) had a basal [K⁺]_out of 4.34 ± 0.01 mM, similar to that of bathing aCSF. Antidromicstimulation (1 Hz for 4 min) induced a transient elevation of[K⁺]_out to ~5 mM; recovered to baseline values within the fourthminute of stimulation (n = 4). During the following stimulationat 0.05 Hz, [K⁺]_out transiently decreased to ~4 mM, and then recovered to baseline.Post-FPI slices (open circles) showed an elevated basal [K⁺]_out during the initial stimulation at 0.05 Hz (4.78 ± 0.08 mM;n = 4). When the 1 Hz stimulation protocol was applied, [K⁺]_out transiently increased to ~5.4 mM and then declined to 5 mM(5 ± 0.05 mM) without reaching its original pre-1 Hz baselinevalue (p < 0.001). During the subsequent stimulation at 0.05 Hz,[K⁺]_out transiently decreased to ~4.7 mM and then recovered to theoriginalbaseline.

These results suggest that the mechanisms responsible for extracellular K⁺ homeostasis are impaired after traumatic injury. Consistent withthat view, we observed that a higher percentage of post-FPI slicesdeveloped burst discharges during the 1 Hz stimulation protocol(Fig. 7B). Only a small fraction of control slices exhibited hyperexcitabledischarges during antidromic 1 Hz stimulation (28%; two of sevenslices), but 80% of post-FPI slices (8 of 10 slices) showed suchactivity.

The abnormal extracellular K⁺ homeostasis is caused by post-traumatic glial impairment

The enhanced accumulation of extracellular K⁺ during 1 Hz stimulation in post-FPI slices could have been caused either by exaggeratedrelease of K⁺ from abnormally hyperactive post-traumatic neurons, to a decreaseduptake of K⁺ by glia, or to a cooperation of both mechanisms. To resolve thisissue, we carried out the same stimulation protocol but in thepresence of the ionotropic glutamatergic receptor antagonist kynurenicacid to block excitatory synaptic drive in CA3 pyramidal cells(Fig. 8). Blockade of glutamatergic synapses with kynurenic acid(1 mM) blocked synaptic excitation in CA3 via axon collaterals(Fig. 8A) and abolished the activation of feedback interneurons(the activity of which could also be altered after FPI). Underthese conditions, none of the slices bathed in kynurenic acid(control and FPI) developed burst discharges when SC were stimulatedat frequencies ranging from 0.05 to 3 Hz, for 4-15 min. We thenapplied Cs⁺ (1 mM) to control slices to block the influx of K⁺ into glia (Janigro et al., 1997; McKhann et al., 1997; D'Ambrosioet al., 1998). Because bath application of Cs⁺ also blocks neuronal h-type currents (Halliwell and Adams, 1982)and modifies neuronal excitability (Maccaferri et al., 1993; Maccaferriand McBain, 1996; Janigro et al., 1997), these experiments wereperformed in the presence of the selective blocker of h-type currentsZD 7288 (10 µM; BoSmith et al., 1993; Gasparini et al., 1996;Gasparini and DiFrancesco, 1997). The application of this selectiveblocker prevented the effect of Cs⁺ on I_h, which would confound the effect of Cs⁺ on glial inward currents, without substantially modifying theprofile of K⁺ accumulation in the extracellular space.

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Figure 8. Abnormal accumulation of extracellular potassium is caused by impaired glial homeostasis. Field electrode and KSM were placed in CA3 stratum pyramidale. Stimulating electrode was placed in CA2 stratum radiatum (A, bottom drawing). Baseline values were obtained at 0.05 Hz stimulation. Bath application of kynurenic acid (1 mM) abolished recurrent spikes (A, top traces; asterisk, artifact of the stimulus). Experiments were performed with bath application of kynurenic acid (1 mM) and ZD 7288 (10 µM), and only slices that had stable population spike and [K⁺]_out were used. B, In control slices, 3 Hz antidromic stimulation induced the rise of [K⁺]_out that peaked at 4.9 ± 0.1 mM. At the end of the 5 min period [K⁺]_out was 4.5 ± 0.05 mM. In the following 5 min of stimulation at 0.05 Hz, [K⁺]_out reached the value of at 3.9 ± 0.1 mM (n = 3). C, Cs⁺ (1 mM) added to the control bath solution increased baseline [K⁺]_out to 4.9 mM. Three hertz antidromic stimulation induced the rise of [K⁺]_out to 5.2 ± 0.1 mM. At the end of the 5 min period [K⁺]_out was still 5.2 ± 0.1 mM. In the following 5 min of stimulation at 0.05 Hz, [K⁺]_out reached the minimum value of 4.7 ± 0.05 mM (n = 3). D, In post-FPI slices, 3 Hz antidromic stimulation induced the rise of [K⁺]_out that peaked at 5.2 ± 0.1 mM. At the end of the 5 min period [K⁺]_out was 5.1 ± 0.1 mM. In the following 5 min of stimulation at 0.05 Hz, [K⁺]_out reached the value of at 4.7 ± 0.05 mM (n = 3).

For this set of experiments, field recordings were paired to concomitant extracellular K⁺ activity recordings in CA3 stratum pyramidale. Baseline valuesof [K⁺]_out and of the population spike amplitude were recorded for 5min during SC stimulation at 0.05 Hz. In slices that had stablepopulation spike and extracellular K⁺ activity for at least 5 min, we then antidromically activatedCA3 with SC stimulation at 3 Hz for 5 min. In control slices,this protocol induced a transient increase of [K⁺]_out that peaked at 4.9 ± 0.2 mM and recovered to 4.5 ± 0.1 mM(n = 3) at the end of the 5 min period. In the ensuing 5 min ofstimulation at 0.05 Hz, there was an undershoot of [K⁺]_out of 0.45 ± 0.05 mM, reaching the value of 3.9 ± 0.1 mM (Fig.8B). After a 30 min recovery period, 1 mM Cs⁺ was added to the bathing solution containing ZD 7288 and kynurenicacid. Ten minutes of Cs⁺ perfusion established a new baseline of [K⁺]_out at 4.9 ± 0.1 mM. Five minutes of 3 Hz antidromic activationunder these conditions induced a persistent increase of [K⁺]_out (5.2 ± 0.1 mM). At the end of the 5 min period, [K⁺]_out was consistently elevated (5.2 ± 0.1 mM; n = 3). In the following5 min of stimulation at 0.05 Hz, an undershoot of [K⁺]_out of 0.2 ± 0.05 mM (significantly smaller than that observedin absence of Cs⁺; p < 0.01) occurred to a value of 4.7 ± 0.05 mM (Fig. 8C).

These same experiments were performed in slices obtained from post-FPI animals. As in control slices, bath application ofZD 7288 and kynurenic acid prevented the appearance of afterdischarges.Five minutes of 3 Hz CA3 antidromic stimulation induced an increaseof [K⁺]_out that peaked at 5.2 ± 0.1 mM and did not recover toward baselinevalues (similar to control slices bathed in 1 mM Cs⁺; Fig. 7). At the end of the 5 min period, [K⁺]_out was 5.1 ± 0.1 mM (n = 3). The following 5 min of stimulationat 0.05 Hz we observed an undershoot of [K⁺]_out of 0.15 ± 0.05 mM that was significantly smaller than thatobserved in control (p < 0.01) and comparable to that in Cs⁺-treated slices (p = 0.6). The undershoot reached a [K⁺]_out of 4.7 ± 0.05 mM (Fig. 8D). Neuronal activity was monitoredthroughout the experiment, and no abnormal synchronous firingwas observed. These results suggest that abnormal accumulationof extracellular potassium during sustained neuronal firing occurseven in the absence of enhanced released of K⁺ from post-traumatic hyperactiveneurons.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To our knowledge this is the first report demonstrating impairment of glial potassium homeostasis in post-traumatic hippocampus.The present study takes advantage of a clinically relevant invivo model of TBI (Dixon et al., 1987), combined with the studyin acutely isolated hippocampal slices. This approach allows usto study at the single-cell level the events accompanying thepathological progression of TBI in vivo. We have asked whetherpost-traumatic electrophysiological changes in hippocampal gliacan promote abnormal neuronal function and have focused on theCA3 subregion of the hippocampus for our analysis. FPI inducesreactive gliosis in this hippocampal region, as well as significantelectrophysiological changes in CA3 glia. Trauma was associatedwith loss of inwardly rectifying and transient outward potassiumcurrents. Furthermore, post-FPI slices exhibited elevated baseline[K⁺]_out and altered neuronal activity-induced extracellular K⁺ accumulation; the latter did not appear to be caused by enhancedK⁺ release from neurons. The results suggest that post-FPI gliain CA3 have impaired uptake of potassium. These findings parallelnumerous reports describing post-traumatic neuronal remodelingleading to hyperecitability and present a new non-neuronal processthat can contribute to post-traumatic changes in neuronalfunction.

Properties of post-FPI hippocampal glia

Despite the loss of inwardly rectifying K⁺ current in post-traumatic glia, their RMPs did not differ significantly from controlvalues. This result is consistent with our previous finding innormal tissue, that there were no differences in RMPs among thethree types of glia differently endowed with Cs⁺-sensitive inwardly rectifying K⁺ currents (D'Ambrosio et al., 1998b). At least two possibilitiesexist: (1) post-FPI glia express Cs⁺-insensitive conductance regulating RMP; or (2) the Cs⁺-sensitive inwardly rectifying channels do not contribute significantlyto the RMP recorded at the cell soma because they are locatedin the fine distal processes. Although reactive glia have beenassociated with depolarized RMPs (MacFarlane and Sontheimer, 1997;Bordey and Sontheimer, 1998), Burnard et al. (1990) found unalteredRMPs in reactive glia in hippocampal slices from kainic acid-treatedrats. Further experiments are thus required to clarify thisissue.

No changes in R_IN measured around RMP were observed in post-FPI reactive glia. This may depend on the distal sites of theinwardly rectifying channels that cannot be probed by the protocolused to test R_IN. Indeed, because of poor space-clamp associatedwith recordings from cells with highly intricate morphology, voltagesteps of ±5 mV applied to the glial cell soma are not likely toinfluence the membrane potential of fine distal processes wherethe channels are likely to be predominantly located (Mi et al.,1996). That changes in membrane conductance occur after lesionwas confirmed when the cell soma was voltage-clamped at significantlymore negativepotentials.

There was a dramatic decrease in membrane capacitance of complex cells after FPI. Interestingly, all complex cells showedoligodendrocyte-like morphology at the light microscope level.Since these cells showed no cell-to-cell coupling even in normaltissue (D'Ambrosio et al., 1998b), we interpret the loss of capacitancenot as a result of uncoupling, but rather as a disruption of cellprocesses. This disruption may have consequences on the K⁺ homeostasis in the region of the axons ensheathed by those oligodendroglia,modifying axonal excitability and conduction. Indeed, it has beensuggested that oligodendroglia and Schwann cells are capable ofpassive K⁺-uptake through ion channels in corpus callosum and spinal cord(Chvátal et al., 1997, 1998), and at peripheral nodes of Ranvier(Mi et al., 1996).

After FPI, complex and inward rectifier cells experienced a loss of Cs⁺-sensitive inwardly rectifying K⁺ currents (Figs. 3, 4). This finding is consistent with previousreport by others showing loss of inward K⁺ currents in reactive glia from human epileptic foci (Bordey andSontheimer, 1998) or in an in vitro model of injury-induced reactivegliosis (MacFarlane and Sontheimer, 1997). The inward rectifierK⁺ current provides an efficient passive mechanism for bufferingextracellular K⁺ (Newman, 1984, 1995) and contributes to K⁺ influx into hippocampal glia in situ (D'Ambrosio et al., 1998b).In addition to loss of inward K⁺ currents, complex cells had a dramatic loss of transient outwardcurrents; because this current is activated by depolarizations,it could contribute to RMP maintenance after changes in extracellularK⁺ and thus be involved in K⁺ homeostasis (Chvátal et al., 1997, 1998).

The observation of post-traumatic changes of glial K⁺ conductances that are active at RMP have led us to conclude that post-traumaticglia have impaired passive uptake of K⁺ through ion channels. This impairment would occur whether K⁺ buffering is accomplished by the spatial buffer mechanism orby passive influx of KCl through ion channels (Newman, 1995).

Abnormal extracellular K⁺ accumulation occurs in post-FPI hippocampus

Because glial K⁺ channels are involved in ion homeostasis, one would predict that post-FPI-mediated loss of K⁺ conductances would have functional effects similar to drug-mediatedblockade of these conductances in normal slices. Because Cs⁺ treatment blocks those channels and leads to an alteration in[K⁺]_out regulation and neuronal excitability, we investigated thesefeatures in post-FPIslices.

Whereas in CA3, control slices exhibited baseline [K⁺]_out equivalent to the [K⁺] in medium bathing the tissue, post-FPI CA3 had a baseline [K⁺]_out that was ~0.5 mM higher. Albeit small, this difference issignificant and can affect hippocampal function. In fact, it hasbeen shown that CA3 pyramidal cell firing is exquisitely sensitiveto small changes of [K⁺]_out (Jensen et al., 1994). Furthermore, our measure is likelyto be an underestimate of the actual increase in baseline [K⁺]_out occurring in vivo after FPI because removal of K⁺ is facilitated by bath flow in the hippocampal slice in vitro.

We chose to study the efficacy of [K⁺]_out regulation during neuronal activity by antidromically activating CA3 pyramidal cells.This approach bypassed the likely involvement of the hilar neuronalnetwork that is affected by FPI (Lowenstein et al., 1992; Gradyet al., 1996). In control slices, 1 Hz stimulation induced a transientincrease of [K⁺]_out that returned to baseline toward the end of the 4-min-longstimulation protocol. However, in post-FPI slices, [K⁺]_out did not return to baseline during this time period, exhibitinga much longer time course recovery. These post-FPI slices werealso more prone to burst discharge generation than control slicesduring this stimulation protocol, suggesting that CA3 pyramidalcell excitability is abnormal at a time when regulation of baseline[K⁺]_out, and of neuronal-activity-induced K⁺ accumulation, is impaired. In a previous study, we found thatpost-FPI CA1 pyramidal cells are hypoexcitable when orthodromicallystimulated. We assessed this change in excitability as higherstimulating currents required to evoke the postsynaptic fieldEPSP and population spike response (D'Ambrosio et al., 1998a).We didn't perform similar experiments in the present study becausewe were interested in the generation of burst discharges afterpurely antidromic population spikes, and antidromic stimulationwas performed to avoid confounding effects of post-traumatic changesin synaptictransduction.

Abnormal accumulation of extracellular K⁺ is caused by impaired glial K⁺ homeostasis

However, the above mentioned experiment does not directly address the question whether the glial impairment is contributingto the abnormal neuronal stimulation-induced extracellular K⁺ accumulation. Indeed, both enhanced neuronal firing and abnormalglial function could result in greater amounts of K⁺ accumulated in the extracellular compartment. A dissociationbetween the neuronal and the glial contribution is difficult toestablish, and has therefore delayed our understanding of therole of glia in [K⁺]_out regulation. Almost 30 years ago, Pollen and Trachtenberg(1970) hypothesized a critical role for reactive glia in abnormalneuronal function through impairment of K⁺ homeostasis. However, without control of neuronal excitability,the central role of glia malfunction could not be determined (Glötzner,1973; Pedley et al., 1976; Lewis et al., 1977).

We investigated this issue by taking advantage of pharmacological manipulations allowed by the hippocampal slice preparation.CA3 recurrent synaptic excitation was abolished by bath applicationof kynurenic acid (1 mM), thus preventing burst discharges inall slices (whether obtained from control rats or from post-FPIrats). Using a combination of the I_h-selective blocker ZD 7288(BoSmith et al., 1993; Gasparini et al., 1996; Gasparini and DiFrancesco1997) and Cs⁺, we selectively targeted the influx of K⁺ through glial ion channels. Furthermore, potassium currents throughion channels cannot be inward in neurons because the average neuronalRMP (approximately $-$ 60 mV) is much more depolarized than E_K (approximately $-$ 90 mV) (Hille, 1993). Under these experimental conditions innormal slices (i.e., in the presence of Cs⁺) baseline [K⁺]_out increased to 4.9 mM, similar to baseline values after FPI.During 3 Hz stimulation, potassium levels peaked at 5.2 mM anddid not return to baseline values (and there was almost no undershootwhen the 0.05 Hz stimulation was restored), again, similar tothe K⁺ response in post-FPI slices. Thus, extracellular Cs⁺ in normal slices reproduced the impairment of K⁺ regulation observed in post-FPI slices, under a condition inwhich network excitability in neurons was not a contributingfactor.

Conclusions and implications

It has been long suspected that reactive glia may have improper K⁺-buffering capabilities (Pollen and Trachtenberg, 1970), and ithas been observed that glial reactivity is accompanied by lossof inward K⁺ current (Francke et al., 1997; MacFarlane and Sontheimer, 1997;Bordey and Sontheimer, 1998). However, the question of whetherreactive glia in general, and post-traumatic glia in particular,are capable of adequate ion homeostasis has not been directlyaddressed. We have now shown that 2 d after FPI neuronal functionis altered, and that the resultant hyperexcitability is causedby an impairment of K⁺ homeostasis that follows the loss of glial K⁺ conductances. This finding may be relevant to an understandingof learning and memory impairments, or seizure susceptibility,that can follow TBI. In fact, each of these neurological deficitscan be caused by altered CA3 pyramidal cell excitability (Traynelisand Dingledine, 1988; Thompson, 1991; Hetherington and Shapiro,1997). Our results provide evidence of the functional consequenceof the loss of K⁺ inwardly rectifying currents in reactive glia and add an additionallevel of complexity to the interplay of mechanisms that are involvedin the development of neurological disorders afterTBI.

  FOOTNOTES

Received Feb. 18, 1999; revised June 14, 1999; accepted July 7, 1999.

This work was supported by a grant from the Epilepsy Foundation (R.D.) and by National Institutes of Health Grants NIEHS ES07033, NS 18895, NS 51614 (D.J.), and NS 33107 (M.S.G.). We wouldlike to thank W. Shawn Carbonell for proofreading, and Guy M.McKhann II and Philip A. Schwartzkroin for helpful comments andreview of this manuscript. We are also grateful to Lesnick E.Westrum and H. Jurgen Wenzel for help with the cameralucida.
Correspondence should be addressed to Dr. Damir Janigro, Cleveland Clinic Foundation NB20, Neurosurgery, 9500 Euclid Avenue/DeskS80, Cleveland, OH44195.

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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