Post-Traumatic Hyperexcitability Is Not Caused by Impaired Buffering of Extracellular Potassium

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The Journal of Neuroscience, July 2, 2003, 23(13):5865-5876

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Post-Traumatic Hyperexcitability Is Not Caused by Impaired Buffering of Extracellular Potassium
Vijayalakshmi Santhakumar,¹ Juha Voipio,² Kai Kaila,² and Ivan Soltesz¹
¹Department of Anatomy and Neurobiology, University of California, Irvine, California 92697-1280, and ²Department of Biosciences, University of Helsinki, 00014 Helsinki, Finland

   Abstract

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Impaired extracellular potassium buffering has been proposedas one of the major mechanisms underlying the increased riskfor temporal lobe epilepsy after brain injury (D'Ambrosio etal., 1999). The present study systematically tested this hypothesisby measuring the resting [K⁺]_o and recovery of the stimulation-evoked[K⁺]_o increases in the dentate gyrus after experimental headtrauma, using a combination of whole-cell recordings and ion-selectivemicroelectrode recordings in rat hippocampal slices. Despite the presence of hyperexcitability, the resting [K⁺]_o was notincreased after injury. The faster rate of increase and largeramplitude of the orthodromically evoked [K⁺]_o elevation afterhead trauma occurred in association with a greater populationspike with shorter response latency. Contrary to the assumptionin previous studies that the evoked activity in control andinjured neuronal circuits is the same during antidromic activation,stimulation of granule cell axons in glutamate receptor antagonistsevoked a greater [K⁺]_o increase and a larger population spike.Although perforant path stimulation resulted in a larger [K⁺]_oelevation after injury, the rate of clearance of the [K⁺]_otransients evoked either by neuronal activity or by externalapplication of potassium was not compromised. The [K⁺]_o increaseevoked by activation of the presynaptic afferents in isolationwas not increased. In addition, the postsynaptic neuronal depolarizationand firing evoked by exogenous potassium application was decreasedafter trauma.
These results show that the regulation of [K⁺]_o is not impairedafter injury and indicate that the larger [K⁺]_o increase evokedby neuronal activity is a consequence, rather than the primarymechanism underlying post-traumatic hyperexcitability.

Key words: potassium; buffering; head trauma; FPI; dentate gyrus; seizures

   Introduction

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Head injury is an important risk factor in the etiology of temporallobe epilepsy (Jennett, 1975; Annegers and Coan, 2000). Althoughconcussive brain trauma causes a distinct pattern of cellularinjury in the dentate gyrus (Margerison and Corsellis, 1966;Bruton, 1988), the exact mechanisms that underlie the postinjuryonset of seizures are unknown.
An intriguing hypothesis suggests that elevated extracellularpotassium ([K⁺]_o) is the key to post-traumatic hyperexcitability and seizures (D'Ambrosio et al., 1999). The impaired potassiumbuffering theory proposes that [K⁺]_o increases, as a consequenceof impaired glial clearance, cause neuronal hyperexcitability (Pollen and Trachtenberg, 1970; D'Ambrosio et al., 1999).Consistent with the contribution of [K⁺]_o to neuronal activity (Huxley and Stampfli, 1951), conditions that disrupt [K⁺]_oregulation by artificially elevating [K⁺]_o (Traynelis andDingledine, 1988; Helekar and Noebels, 1992; McBain et al., 1993) or by manipulations that depress glial K⁺-uptake (Largoet al., 1996; Janigro et al., 1997; Xiong and Stringer, 1999)can cause neuronal hyperexcitability. Recent data demonstratingpostinjury reduction in glial inward rectifier potassium currents(K_IR) that are thought to regulate [K⁺]_o, and the abnormal [K⁺]_o increases evoked by antidromic stimulation in glutamatereceptor antagonists in vitro, a paradigm assumed to normalizeneuronal activity between injured and control tissue, were presented as evidence that supported the glial impairment theory (D'Ambrosioet al., 1999). However, studies have shown that the immediatepost-traumatic increase in resting [K⁺]_o in vivo recovers tocontrol levels within a few hours (Takahashi et al., 1981;Katayama et al., 1990). Similarly, regulation of both the resting [K⁺]_o and the activity-dependent [K⁺]_o increases is not compromisedin electrically induced seizure foci (Xiong and Stringer, 1999). In addition to the controversy concerning the glial impairment theory (Walz and Wuttke, 1999), results demonstratingthat [K⁺]_o elevations often follow, rather than precede, seizure-likeactivity in animal models of epilepsy (Pedley et al., 1976;Somjen, 1984) call into question the role for altered [K⁺]_oregulation as a major mechanism for seizure generation.
The dentate gyrus regulates the neuronal signaling between theentorhinal cortex and the hippocampus (Buzsaki et al., 1983)and has been proposed to gate seizure propagation in the limbicsystem (Heinemann et al., 1992; Lothman et al., 1992). Itis also the site of characteristic post-traumatic alterations,including hilar cell loss (Lowenstein et al., 1992; Coulteret al., 1996; Toth et al., 1997), mossy fiber sprouting (Golaraiet al., 2001; Santhakumar et al., 2001), and reactive gliosis (Smith et al., 1997). Furthermore, studies investigating neuronalexcitability using the rodent fluid percussion head injury(FPI) model of concussive head trauma have demonstrated neuronalhyperexcitability (Lowenstein et al., 1992; Coulter et al.,1996; Toth et al., 1997) and modifications in the dentateinterneuronal and excitatory networks (Ross and Soltesz, 2000; Santhakumar et al., 2000; Ratzliff et al., 2002). Despitethe data that imply that the changes in the dentate gyrus mightbe pivotal to seizure generation (Coulter et al., 1996; Masukawaet al., 1999; Santhakumar et al., 2001), little is known aboutthe efficacy of [K⁺]_o regulation in the dentate after headinjury.
This study was performed to test the hypothesis (D'Ambrosioet al., 1999) that an impaired regulation of the resting [K⁺]_oand the stimulation-evoked [K⁺]_o transients underlies posttraumatichyperexcitability.

   Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Fluid percussion injury. Lateral fluid percussion head traumaon young adult (4 weeks of age) male Wistar rats was carriedout as described previously (Dixon et al., 1987; Lowensteinet al., 1992; Toth et al., 1997) (all procedures describedwere approved by the Institutional Animal Care and Use Committee,University of California, Irvine, CA). Briefly, the rats wereanesthetized, placed in a sterotaxic frame, and the scalp was sagittally incised. A 2 mm hole was trephined in the skull at-3 mm (i.e., caudal) from the bregma, 3.5 mm lateral from thesagittal suture. A Luer-Loc syringe hub with a 2.6 mm insidediameter was placed over the exposed dura and bonded with cyanoacrylateadhesive. A day later, the rats were anesthetized with halothanein a 2 liter chamber and subsequently removed from the anesthetizingchamber and immediately connected to the injury device. The animal was fully anesthetized at the time of injury, althoughhalothane anesthesia was not actively administered at thattime. All animals were immediately ventilated with room air.The fluid percussion device (Department of Biomedical Engineering,Virginia Commonwealth University, Richmond, VA) was used toinject a small volume of saline into the closed cranial cavityon the intact dura and produce a brief (20 msec) displacementand deformation of the brain tissue. The magnitude of the injurywas controlled by varying the height from which the pendulumin the injury device was released (in these experiments, itwas 12–14°, which produced a 2.0–2.2 atm pressurewave). This resulted in a moderate level of injury that hasbeen shown to cause a highly reproducible pattern of >50%hilar cell loss (Toth et al., 1997; Santhakumar et al., 2000).
Slice preparation. At various time points (2 d, 1 week, and1 month) after the injury, or sham injury (Toth et al., 1997),the rats were anesthetized with halothane and decapitated.Horizontal brain slices (400 µm) were cut using a vibratometissue sectioner (VT1000S; Leica, Nussloch, Germany), as describedpreviously (Ross and Soltesz, 2001). The slices were sagittallybisected, and the slices ipsilateral to the side of injurywere submerged in 32°C oxygenated (95% O₂-5% CO₂) artificialCSF (ACSF) composed of (in mM): 126 NaCl, 2.5 KCl, 2 MgCl₂,26 NaHCO₃, 2 CaCl₂, 1.25 NaH₂PO₄, and 10 glucose, for 1–6hr.
In vitro electrophysiology. The slices were transferred to the interface recording chamber and perfused with oxygenated ACSFat 36°C. In some experiments, the perfusion was switchedto ACSF containing one or more of the following drugs: 20 µMbicuculline methiodide (BMI), 20 µM D-AP-5, 10 µMCNQX, 100 µM picrotoxin, 10 µM 2,3-dioxo-6-nitro-1,2,3,4-tetrahydrobenzo[f]quinoxaline-7-sulfonamide(NBQX), 20 µM (2S)(+)5,5-dimethyl-2-morpholineaceticacid (SCH 50911), 500 µM (RS)-a-methyl-4-carboxyphenylglycine(RS-MCPG), and 1 µM TTX. All salts were obtained fromFluka (Buchs, Switzerland). AP-5, CNQX, NBQX, picrotoxin, RS-MCPG,SCH 50911, and TTX were purchased from Tocris (Bristol, UK);QX-314 was obtained from Calbiochem (La Jolla, CA); and BMIfrom Sigma--Research Biochemicals International (Natick, MA).
Single-barrel ion-selective microelectrodes (ISME) were silanized, backfilled with 3 mM KCl, and the tip was filled with valinomycin-basedmembrane solution selective for potassium ions (Cocktail B; Fluka; Voipio et al., 1994). Signals from the ISMEs were recordedusing a custom-built electrometer amplifier that has a biascurrent of <50 fA, an input impedance three orders of magnitudehigher than the electrode resistance, and a feedback circuitfor electrode capacitance compensation. The ISMEs (1–10 G ${Omega}$ ) were calibrated using solutions containing 2.5, 5, and 10 mM potassium. Only electrodes with a slope in the range of 54–60 mV/10-fold change in [K ⁺] were used. The ISME capacitance was compensated using the feedback circuit of theamplifier. A double electrode holder (Narishige, Tokyo, Japan)was used to position the ISME and a reference electrode ata constant tip separation of 5 µm. Field potential recordingswere obtained using the reference electrode coupled to theISME. The field responses and [K ⁺]_o measurements were obtainedfrom the crest of the dentate granule cell layer at a depthof 150 µm from the surface of the tissue. Level-matchedslices from head-injured and age-matched sham-operated controlanimals were recorded alternately on the same day. Orthodromicpopulation spikes in granule cells were evoked by constant–currentstimuli (1–8 mA, 50 µsec) at 0.1 Hz using a bipolartungsten-stimulating electrode placed in the perforant path,on the entorhinal side of the fissure, at the junction of thedorsal blade, and at the crest. Control experiments conductedin the absence of the slice showed that stimulation in thebath did not induce an artifactual ion–electrode signal(n = 6). For antidromic activation of granule cells, the stimulatingelectrode was located in the hilus, halfway between the tipof the upper blade and the crest of the granule cell layer, and midway between the granule cell layer and CA3 (at $~$ 60–70µm from the recording electrode), and the slices wereperfused with ionotropic glutamate and GABA receptor antagonists(20 µM AP-5, 10 µM CNQX, and 20 µM BMI; or20 µM AP-5, 10 µM NBQX, and 100 µM picrotoxin). Similarly, CA3 cells were stimulated antidromically by an electrodeplaced in the Schaffer collaterals in 20 µM AP-5, 10µM CNQX, and 20 µM BMI. Either single-shock stimuli(1–6 mA, 50 µsec) at 0.1 Hz or 50 msec trains of5–10 stimuli (at 100–200 Hz) at 6 mA stimulationintensity were used to evoke antidromic firing. Tetanic stimulationconsisted of a 5 sec, 100 Hz train of stimuli applied to theperforant path with a pulse width of 0.1 msec at 8 mA stimulus intensity. Exogenous potassium was applied using a glass pipettewith a 10 µm diameter tip opening, containing ACSF witheither 10 or 120 mM potassium (replacing potassium for equimolarsodium to maintain osmotic balance). The potassium applicationpipette was placed in the bath (with the tip above the surfaceof the slice) on the hilar side of the granule cell layer 20µm (for experiments shown in Fig. 3) or 50 µm (for experiments shown in Fig. 7) from the recording electrode.In separate experiments (similar to those in Fig. 7), pressureapplication of ACSF containing 120 mM potassium for 10 msecwas found to cause over a 6 mM increase in potassium at a depthof 250 µm in the granule cell layer (n = 3 slices). Apressure ejection pump (Picospritzer) was used to apply thepotassium solution at 4–8 psi. Representative tracesof [K ⁺]_o transients are plotted as voltage changes from theISME recordings, and the corresponding [K ⁺]_o (as a micromolarincrease from resting [K ⁺]_o; calculated from the mV changefrom rest) is indicated on a Nernstian scale. For simplicity,the summary data in bar graph form show the relative increasein [K ⁺]_o (in mM) above the resting [K ⁺]_o on a linear scale.Blind whole-cell recordings were obtained as described previously (Toth et al., 1997; Santhakumar et al., 2000; Chen et al.,2001), using patch pipettes filled with an internal solutionthat consisted of (in mM) 140 K-gluconate, 2 MgCl₂, and 10HEPES. The correction for the junction potential was not performed.The sodium and nonspecific potassium channel blocker QX-314(3 mM) was included in the internal solution in some experimentssummarized in Figure 7.

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Figure 3. The rate of clearance of externally applied potassium is not impaired after head injury. A, Example of traces showing [K ⁺]_o elevation and clearance in the granule cell layer during pressure application of ACSF containing 10 mM potassium in 1µM TTX 1 week after injury (FPI) or sham operation (CON) (the y-axis showing [K ⁺]_o elevation above rest as a micromolar concentration is on a Nernstian scale). B, C, Summary data showing no difference in the either the fast (B) or the slow (C) exponential decay time constants of the externally applied potassium between slices from injured and control animals.

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Figure 7. Post-traumatic decrease in granule cell firing in response to exogenous application of potassium. A, Representative voltage traces from granule cells in control animals (CON) and head-injured animals (FPI) show the post-traumatic decrease in depolarization and action potential firing evoked by exogenous potassium application. The traces were obtained by whole-cell patch-clamp recordings at -70 mV in 20 µM BMI, 20 µM AP-5, and 10 µM CNQX, 1 week after FPI. B, Summary data show the smaller potassium-evoked depolarization of granule cells from head-injured animals compared with controls from experiments similar to those in A. Inset in B shows that the difference in the potassium-induced depolarization was absent when QX-314 was present in the internal solution of the recording whole-cell pipette. C, Granule cell I/V plots from control animals ( ${bullet}$ ; n = 5) and head-injured animals ( ${circ}$ ; n = 5) show that that there was no discernable difference in the voltage response evoked by +50 pA to -400 pA current steps (from a holding potential of -70 mV) after head trauma. Inset, Granule cell I/V plots from a subset of the cells, from control animals ( ${bullet}$ ; n = 3) and injured animals ( ${circ}$ ; n = 3) in C in which larger current steps could also be tested, show that that there was no difference in the voltage response evoked by +50 pA to -700 pA current steps after head trauma.

Analysis. Recordings were filtered at 3 kHz and digitized at20 kHz using the Strathclyde Electrophysiology software (courtesyof Dr. J. Dempster, University of Strathclyde, Glasgow, UK)and Synapse software (courtesy of Dr. Y. De Koninck, McGillUniversity, Montreal, Canada). Half-time of recovery of [K⁺]_o transients, a measure of the rate of potassium clearance,was defined as the time taken for [K ⁺]_o to decline to half-maximumamplitude (Xiong and Stringer, 1999). To assess whether thedecay of the [K ⁺]_o transients was better fit with single ordouble exponentials, the sum of squared errors (SSE) improvementfunction (Hollrigel et al., 1996; Chen et al., 2001) was used.Briefly, an F-test was used to assess the improvement in theratio (SSE₁-SSE₂)/SSE₂ where SSE₁ and SSE₂ are the sum of squarederrors of fits with one and two exponentials. When SSE improvementwas not significant, a single exponential described the decay.Statistical analyses were performed with SigmaPlot or SPSSfor Windows (SPSS, Inc., Chicago, IL). The significance ofdifferences in field and whole-cell responses and [K ⁺]_o changesin control and injured animals was evaluated using the Student'st test. The Mann–Whitney U test was used to assess thesignificance of differences in [K ⁺]_o increase in responseto tetanic stimulation. The statistical significance of changesin potassium-evoked firing was tested using the nonparametricz-test. The level of significance was set at p < 0.05. Dataare presented as mean ± SEM.

   Results

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Absence of increase in the resting [K⁺]_o after head trauma
It has been reported previously that the resting [K⁺]_o in hippocampalslices is significantly elevated after FPI (D'Ambrosio et al., 1999). The study by D'Ambrosio et al. (1999) was conductedin CA3 2 d after head injury. The present study examined theresting [K⁺]_o in the dentate gyrus at various time points after head trauma. Additionally, the resting [K⁺]_o was also measuredin the CA3 pyramidal cell layer 2 d after injury to facilitate comparison with previous results (D'Ambrosio et al., 1999).
The resting [K⁺]_o was measured in the absence of external stimulationin slices from injured and control animals in which we establishedthe presence of post-traumatic neuronal hyperexcitability. The perforant path-evoked population spike amplitude (Fig. 1A,B)in the animals used in the present study was larger 1 weekafter FPI (Fig. 1A,B), in agreement with the results of earlierstudies (Lowenstein et al., 1992; Toth et al., 1997; Santhakumaret al., 2000). However, the resting [K⁺]_o in the granule celllayer of slices from head-injured animals measured in controlACSF was not increased at the same time point (Fig. 1C) [CON:100 ± 3.3%, n = 16; FPI: 97.94 ± 3.13%, n = 18;for easier comparison, the data are presented as percentageof control, i.e., normalized to control mean; the absolute [K⁺]_o was 2.70 ± 0.09 mM (CON) and 2.64 ± 0.08mM (FPI)]. Similar to the results at 1 week, the resting [K⁺]_oin the dentate gyrus was not different from controls either2 d or 1 month after head trauma (Fig. 1D) (2 d: CON, 100± 0.68%, n = 12; FPI, 100.13 ± 1.57%, n = 12;1 month: CON, 100 ± 3.23%, n = 5; FPI, 99.81 ± 0.81%, n = 5), indicating that an elevation of the resting [K⁺]_o cannot underlie the long-term decrease in seizure threshold(Santhakumar et al., 2001). Consistent with our findings inthe dentate gyrus and in contrast to the results of D'Ambrosioet al. (1999), there was no change in the resting [K⁺]_o inthe CA3 pyramidal cell layer either 2 d (CON: 100 ±2.08%, n = 8; FPI: 96.94 ± 0.71%, n = 8) or 1 monthafter FPI (CON: 100 ± 1.98%, n = 5; FPI: 99.16 ±1.25%, n = 5).

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Figure 1. Resting [K ⁺]_o is not increased in the post-traumatic dentate gyrus. A, Field recordings of perforant path-evoked granule cell responses are shown, 1 week after moderate head injury in slices from a fluid percussion-injured animal (FPI) and an age-matched sham-control animal (CON) in ACSF (at 6 mA stimulation intensity). B, Summary data obtained from experiments similar to those in A. Note that the amplitude of the population spike in slices from head-injured animals is larger than controls, indicating the presence of post-traumatic hyperexcitability. C, The resting [K ⁺]_o in the granule cell layer from the same slices as in B was not increased 1 week after head trauma. D, There was also no increase in the resting [K ⁺]_o 2 d and 1 month after injury. E, Resting [K ⁺]_o in the granule cell layer in 20 µM BMI and 20 µM AP-5 was not different between head-injured and control animals 1 week after FPI. [Inset, Similar results were obtained in 100 µM picrotoxin (Ptx) and 20 µM AP-5.]

Previous results have shown hyperexcitability of the dentateexcitatory circuit (Santhakumar et al., 2000) even when theposttraumatic differences in fast inhibition (Toth et al.,1997) are abolished in the presence of GABA_A receptor antagonists.Therefore, we examined the possible role for resting [K⁺]_oincrease in the neuronal hyperexcitability observed in GABA_Areceptor antagonists (20 µM BMI) 1 week after FPI. Onceagain, there was no postinjury increase in the resting [K⁺]_o,even in BMI and the NMDA receptor antagonist AP-5 (Fig. 1E)[CON: 100 ± 4.41%, n = 10; FPI: 101.02 ± 4.00%,n = 12; note that 20 µM AP-5 was included only to conformto our previous study (2000)]. Additionally, there was no increasein the resting [K⁺]_o after head injury when the GABA_A channelblocker picrotoxin (100 µM) was substituted for BMI (Fig. 1E) (inset; CON: 100 ± 1.13%, n = 7; FPI: 98.46 ±1.12%, n = 9) to control for any potential nonspecific effectsof potassium channel block by BMI (Khawaled et al., 1999) on [K⁺]_o.
Taken together, these data demonstrate that the resting [K⁺]_ois not increased at any time point after injury.
Clearance of stimulation-evoked increases in [K⁺]_o is not impairedafter head injury
The next series of experiments were performed to examine thepost-traumatic changes in the buffering of [K⁺]_o transientsevoked by neuronal activity, in control medium. The rate ofclearance of the tetanic stimulation-evoked [K⁺]_o increaseswas measured in the granule cell layer 1 week after FPI. Asshown by representative [K⁺]_o traces in Figure 2A, the amplitudeof the orthodromically evoked [K⁺]_o elevation (above the resting[K⁺]_o) was larger after head trauma (Fig. 2B) (CON: 0.87 ±0.14 mM, n = 29; FPI: 1.35 ± 0.22 mM, n = 30), suggestingan increase in [K⁺]_o elevation as a result of neuronal hyperexcitabilityor a deficiency in the clearance of [K⁺]_o. Indeed, the granulecell population spike was increased after head trauma, as measuredafter single-shock stimulation of the perforant path (Fig. 2B, inset) (at 8 mA stimulation intensity; CON, 0.51 ±0.04 mV; FPI, 1.06 ± 0.20 mV), suggesting that the enhanced orthodromically evoked neuronal activity might contribute tothe larger [K⁺]_o increase (Fig. 2A,B). In contrast, the half-timeof recovery of the evoked [K⁺]_o transients (time taken forthe [K⁺]_o elevation to decay to half the peak amplitude) was not increased (Fig. 2C) (CON, 5.19 ± 0.89 sec; FPI,5.34 ± 0.33 sec), showing that buffering of the stimulation-evoked [K⁺]_o transients was not compromised. These findings indicatethat increased neuronal firing, and not an impaired bufferingof [K⁺]_o, is likely to underlie the greater [K⁺]_o increaseafter tetanic stimulation of afferents after head trauma.

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Figure 2. Absence of postinjury decrease in the rate of clearance of tetanic stimulation-evoked [K ⁺]_o increase. A, Representative recordings of [K ⁺]_o in the granule cell layer evoked by tetanic stimulation of the perforant path at 8 mA stimulation intensity (for 5 sec at 100 Hz) reveal a larger [K ⁺]_o elevation 1 week after trauma (FPI) compared with controls (CON) (the y-axis shows [K ⁺]_o elevation above resting [K ⁺]_o on a Nernstian scale). B, Summary of data demonstrate an increase in the amplitude of the evoked [K ⁺]_o transient (above the resting [K ⁺]_o) after head injury. The asterisk indicates significance (Mann–Whitney U test). Inset, Summary plot showing that the single-shock, perforant path-evoked population spike amplitude (at 8 mA simulation intensity), from the same slices as in B, was larger after head trauma. C, The half-time of recovery of the tetanus-evoked [K ⁺]_o increase was not prolonged in slices from head-injured animals.

In the experiments described above, the postinjury increasein the orthodromic population spike amplitude (Fig. 2B, inset)is an obvious confounding factor in assessing the rate of clearanceof the stimulation-evoked [K⁺]_o transients (Dietzel and Heinemann,1986). Therefore, we examined the rate of decay of [K⁺]_o transientsevoked by pressure application (see Materials and Methods) ofACSF containing 10 mM potassium (for 4 sec) in the presenceof the sodium channel blocker TTX (1 µM) to block actionpotential firing. As shown by the representative [K⁺]_o recordings (Fig. 3A), potassium application evoked [K⁺]_o increases ofsimilar amplitude head-injured and control tissue (CON: 4.24± 0.49 mM, n = 11; FPI: 3.48 ± 0.43 mM, n = 11).The rate of decay of the [K⁺]_o transient after external applicationof potassium was described by the sum of two exponentials, because the SSE improvement (see Materials and Methods; CON, 65.51 ±28.22%, FPI, 63.30 ± 10.73%) was significant. Importantly,the rate of decay of the externally applied potassium was notdecreased after head trauma (Fig. 3B) ( ${tau}$ _{decay (fast)}; CON,1.53 ± 0.18 sec; FPI, 1.59 ± 0.11 sec) (Fig. 3C)( ${tau}$ _{decay (slow)}; CON, 20.22 ± 3.24 sec; FPI, 24.20± 4.12 sec). Taken together, these data demonstratethat the buffering of [K⁺]_o increases is not impaired afterhead injury.
Larger and faster postinjury increase in orthodromically evoked [K⁺]_o transients
In an effort to determine whether the postinjury increase inthe orthodromically evoked [K⁺]_o transients was a consequenceof the enhanced neuronal activity, we examined the early increase in [K⁺]_o (within 50 msec of stimulation). Because the resolutionof the early time course of [K⁺]_o elevation is difficult whentetanic stimulation is used, the rise and latency of the [K⁺]_oresponses in the dentate granule cell layer were examined inresponse to single-shock perforant path stimulation. The experimentsdescribed in Appendix (available at www.jneurosci.org) andillustrated in Figure 8 established the temporal propertiesof the ISME and made it possible to measure the latency ofthe [K⁺]_o transients evoked by single-shock stimulation.

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Figure 8. Detection of rapid changes in potassium concentration by ISMEs. Representative traces obtained by applying ACSF containing 5 mM (A) or 25 mM (B) potassium for increasing durations (50 msec, 500 msec, 1 sec, and 5 sec)show that brief changes in [K ⁺]_o lasting <500 msec can be detected by ISMEs. C, A schematic of the experimental setup for fast application switch from normal (2.5 mM, white) to high (120 mM, black) potassium concentration is shown. Inset, Regression fit shows the linear time distance profile for the stepping motor operating at 3 µm/msec [see Appendix (available at www.jneurosci.org) for details]. D, Spatial profile of the potassium concentration is shown in the narrow (20µm) interface region between the 2.5 mM and 120 mM potassium flow. Zero on thex-axis indicates the start of the interface region. E, Overlay of the actual and the measured [K ⁺] during the long (i.e., uninterrupted) step from normal to high [K ⁺] across the liquid interface is shown. The trace with circles is the actual K ⁺ concentration outside the electrode tip calculated from the spatial concentration profile of the flow (in D) and the speed of the fast application switch (3µm/msec). The line trace is what the electrode measured during the long step across the liquid interface normal to high [K ⁺]. The inset shows that the electrode correctly measured the change in concentration during prolonged application of 120 mM potassium. F, The first 15 msec of the plots in E shows that a 0.08 mM (equivalent to 0.75 mV) change in [K ⁺]_o can be detected in <4 msec. The top dashed line indicates the threshold level of 0.08 mM increase in [K ⁺]_o, and the bottom dashed line indicates the steady-state [K ⁺]_o.

The amplitude of the single-shock, perforant path-evoked [K⁺]_oresponses and population spikes were measured in the presenceof the GABA_A receptor antagonist BMI (and the NMDA receptorantagonist AP-5), because the orthodromically evoked [K⁺]_otransient in control ACSF could not be resolved above the electricalnoise. As shown in Figure 4A (top traces) and as describedpreviously (Santhakumar et al., 2000), the amplitude of theperforant path-evoked granule cell population spike was enhanced1 week after head injury. In agreement with the larger neuronalfiring, the amplitude of the orthodromically evoked [K⁺]_o transientwas also increased after head trauma (Fig. 4A, middle and bottom traces) (Fig. 4B, [K⁺]_o 50 msec after a 2 mA stimulation)(CON: 0.06 ± 0.01 mM, n = 9; FPI: 0.15 ± 0.03mM, n = 10). Despite the enhanced amplitude, there was no increasein the time constant for exponential decay of the [K⁺]_o transient(Fig. 4C) (CON: 180.28 ± 22.81 msec, n = 4; FPI: 178.62± 35.38 msec, n = 7). Therefore, similar to the resultsof the tetanic stimulation experiments described above, thesedata also suggest that the greater stimulus-evoked [K⁺]_o increaseafter head injury cannot be a result of decrease in the rateof clearance of [K⁺]_o.

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Figure 4. Faster rise and larger amplitude of evoked [K ⁺]_o increase 1 week after head trauma. A, Example traces of granule cell population spikes (top) evoked by perforant path stimulation (stimulation intensity, 2 mA) show the enhanced excitability in BMI (20 µM) and AP-5 (20 µM) after injury (FPI) compared with controls (CON). Representative [K ⁺]_o recordings at the same time scale as the field response (middle) and at a longer time scale (bottom) show a post-traumatic increase in the amplitude of the [K ⁺]_o transient (the scale for micromolar [K ⁺]_o increase is the same for the middle and bottom panels). B, Summary histogram demonstrate a greater evoked [K ⁺]_o increase after head injury, in response to low-frequency perforant path stimulation (at 2 mA). Inset, Summary data show that the presynaptic component of the [K ⁺]_o increase in the granule cell layer, evoked by a train of 10 stimuli (at 6 mA stimulation intensity) in slices recorded in the presence of ionotropic and metabotropic glutamate and GABA receptor antagonists, was not increased after head trauma. C, The exponential decay time constant of single-shock perforant path-evoked [K ⁺]_o transient was not prolonged in slices from head-injured animals. D, Summary bar graphs show the post-traumatic decrease in the latency to a 0.08 mM (0.75 mV) [K ⁺]_o elevation in response to low-frequency stimulation. Inset, Overlay of representative potassium electrode recordings from injured and control animals shows the faster rate of rise and shorter latency to detect a 0.08 mM increase in the evoked [K ⁺]_o elevation after head trauma. The horizontal line indicates a 0.08 mM increase in [K ⁺]_o (0.75 mV depolarization). Calibration bar, 40 msec. E, Histogram demonstrates the postinjury decrease in the rise time constant of the [K ⁺]_o transient. Inset, Summary data show the faster latency to onset of the population spike after head trauma.

After the measurement of the amplitude and decay of the single-shock stimulation-evoked [K⁺]_o elevation, the latency and rise timeswere examined. The early time course of the perforant path-evoked [K⁺]_o transient revealed that the latency to an arbitrary threshold(0.08 mM) increase in [K⁺]_o (Fig. 4D) (CON, 30.94 ±9.12 msec; FPI, 9.67 ± 2.03 msec; see inset for representativetraces), time to peak (CON, 78.37 ± 5.79 msec; FPI,60.22 ± 4.28 msec, n = 7), as well as the time constantfor exponential rise of [K⁺]_o (Fig. 4E) (CON, 33.91 ±3.78 msec; FPI, 20.06 ± 3.07 msec), were significantlyfaster after head trauma. Next, we examined whether an increasein the [K⁺]_o transient evoked by activation of the presynaptic fibers, or a decreased latency to onset of the postsynapticactivity after stimulation of the perforant path fibers, contributedto the faster rise and shorter latency of the orthodromicallyevoked [K⁺]_o increase. The component of the stimulus-evoked[K⁺]_o elevation that was caused by activation of the afferentfibers was determined by perfusing the slices with a mixtureof ionotropic and metabotropic glutamate and GABA antagonists(20 µM BMI, 10 µM CNQX, 20 µM AP-5, 20 µMSCH, and 500 µM RS-MCPG) to block postsynaptic responses.Because the [K⁺]_o elevation in response to a single-shock stimulation of the afferent fibers could not be discriminatedover the electrical noise, a train of 10 stimuli (at 6 mA,200 Hz) was used in these experiments. In agreement with previousstudies demonstrating [K⁺]_o increase by the activation of presynapticfibers (Fisher et al., 1976; Aitken and Somjen, 1986; Jonesand Heinemann, 1987; Poolos et al., 1987), stimulation ofthe perforant path resulted in [K⁺]_o elevations even in theabsence of postsynaptic activity. There was no post-traumaticincrease in the amplitude of the perforant path-evoked [K⁺]_otransient in the presence of blockers of synaptic transmission(Fig. 4B, inset) (peak [K⁺]_o; CON: 0.05 ± 0.01 mM,n = 13; FPI: 0.05 ± 0.01 mM, n = 13), indicating thatan increase in presynaptic [K⁺]_o elevation does not underliethe faster rate of rise of [K⁺]_o after head injury (Fig. 4D,E).As an additional control, we verified that there was no tetanus-evoked [K⁺]_o elevation in the granule cell layer in the presence ofTTX (data not shown), indicating that electrical stimulationcould not directly evoke [K⁺]_o increase in the absence of neuronal activity. In contrast to the lack of difference inthe presynaptic component of the stimulus-evoked [K⁺]_o elevation,both the latency to onset (Fig. 4E, inset) (CON, 2.90 ±0.14 msec; FPI, 2.47 ± 0.08 msec) and the time to peak(CON, 4.33 ± 0.17 msec, FPI, 3.77 ± 0.18 msec)of the single-shock perforant path-evoked postsynaptic populationspike (in BMI and AP-5) were shorter after head trauma. Inagreement with the field recording data, the perforant path-evoked action potential firing, determined in separate experimentsby whole-cell recordings from granule cells (also in BMI andAP-5), occurred at a significantly shorter latency after FPI(CON: 5.13 ± 0.25 msec, n = 4; FPI: 3.83 ± 0.23msec, n = 6; at 4 mA stimulation intensity). However, the latencyto onset of the perforant path-evoked, whole-cell-recordedEPSC in the granule cells was not shorter after injury (CON,1.67 ± 0.05 msec; FPI, 1.89 ± 0.12 msec). Althoughthe mechanisms underlying the decrease in the latency to onsetof firing after trauma are not understood, the main point ofthese results is that the faster rise of [K⁺]_o in responseto single-shock stimulation of the perforant path after headinjury occurs in conjunction with an earlier onset for neuronalactivity, as can be seen in Figure 4A.
These results show that the decay of the [K⁺]_o transient isnot altered by trauma, indicating no alteration in the [K⁺]_obuffering system. Furthermore, these data also demonstratethat the earlier and faster rise of [K⁺]_o does not, by itself,provide evidence for decreased potassium buffering, becauseit occurs in conjunction with an earlier onset of neuronal firing after the activation of the perforant path.
Post-traumatic increase in antidromically evoked [K⁺]_o transients:reexamining protocols that attempt to normalize activity betweeninjured and control neuronal circuits
As demonstrated by the results presented above, it is not possibleto unequivocally establish the cause of the larger [K⁺]_o increasein the traumatized tissue using tetanic or single-shock stimulation of the perforant path, because of the temporal limitations posedby the ISME and the post-traumatic changes in the latency toonset and amount of neuronal firing. However, there is a paradigmthat has been suggested previously to equalize neuronal activityin slices from control and head-injured animals (D'Ambrosioet al., 1999). The experimental protocol is based on antidromicstimulation of the axons in the presence of ionotropic glutamatereceptor antagonists, an approach that is proposed to preciselycontrol principal cell firing. However, this paradigm restson two previously untested assumptions: first, that there isa 1:1 correspondence between the antidromic stimulation andthe firing of action potentials by principal cells; and second,that the antidromic stimulation with a relatively large stimulatingelectrode causes a similar antidromic population spike in bothcontrol and post-traumatic hippocampi.
We implemented this paradigm to examine whether differencesin evoked [K⁺]_o increase were eliminated when the granule cell axons were antidromically stimulated in the hilus. Surprisingly,the amplitude of the [K⁺]_o increase evoked by either trainsof stimuli (Fig. 5A,B) or by a single stimulus (Fig. 5B,top inset) was greater after injury. The larger post-traumaticincreases in the antidromically evoked [K⁺]_o transient couldhave occurred as a consequence of various factors includingan increase in neuronal excitability (Santhakumar et al., 2000),a decrease in the extracellular space that would boost theephaptic field effects (Jefferys, 1995), and/or impaired regulationof [K⁺]_o. Control experiments showed that there was no differencein antidromically evoked [K⁺]_o increase when the perfusatewas switched from a medium containing AP-5, CNQX, and BMI toa solution in which NBQX and picrotoxin were substituted forCNQX and BMI in either the control or injured slices (Fig.5B, bottom inset) (percentage change after perfusate switch;CON: 97.69 ± 19.01%, n = 3; FPI: 104.89 ± 17.84%,n = 3). These data verified that neither the block of certainpotassium channels by BMI (Misgeld et al., 1992; Khawaledet al., 1999) nor an increase in GABAergic currents by CNQX (McBain et al., 1992; Brickley et al., 2001; Maccaferri andDingledine, 2002) affected the amplitude of the measured [K⁺]_otransients in slices from control and head-injured animals.

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Figure 5. Larger antidromically evoked [K ⁺]_o increase after head injury. A, Representative recordings of [K ⁺]_o transients in the granule cell layer evoked by antidromic stimulation at 6 mA (10 stimuli in 50 msec) show the larger [K ⁺]_o elevation in the fluid percussion head-injured animal (FPI) compared with the control (CON), in 20 µM BMI, 20 µM AP-5, and 10 µM CNQX ( ${Delta}$ [K ⁺]_o scale is exponential). Insets, Whole-cell recordings from granule cells in response to 10 stimuli (in 50 msec) show that each hilar stimulus evoked a single action potential in slices from both control and injured animals. Calibration: 20 mV, 10 msec. Recordings were obtained 1 week after head injury. B, Summary data similar to those in A are shown from slices from control animals ( ${bullet}$ ) and FPI animals ( ${circ}$ ), in response to the increasing number of stimuli. Top inset, [K ⁺]_o increase (as a micromolar potassium concentration indicated on the y-axis) in slices from control animals ( ${bullet}$ ) and FPI animals ( ${circ}$ ) animals, evoked by single-shock stimulation in the hilus (see Materials and Methods) at an increasing intensity (indicated on the x-axis in mA). Note that the response to a 6 mA stimulation shown in the inset is the same as the response to a single stimulus in B. Bottom inset, Histograms show the percentage change in the [K ⁺]_o elevation, evoked by a train of 10 stimuli (in 50 msec) to the hilus, when the perfusing medium was switched from 20µM BMI,20µM AP-5, and 10µM CNQXto100µM picrotoxin,20µM AP-5, and 10µM NBQX.C, Fast and slow exponential decay time constants of the antidromically evoked [K ⁺]_o transient were not different between head-injured and control animals 1 week after injury. Inset, The same data as in C, showing that the half-time of recovery of the evoked [K ⁺]_o increase was not prolonged after FPI. D, Half-time of recovery of the antidromic stimulation-evoked [K ⁺]_o transient 2 d and 1 month after FPI was not different from age-matched sham-controls.

Next, the rate of clearance of the antidromically evoked [K⁺]_oincrease was measured, to ascertain whether a post-traumaticdecrease in buffering of [K⁺]_o contributed to the larger [K⁺]_oelevation after head trauma in the experiments described above.The rate of decay of the antidromically evoked [K⁺]_o transientswas better fit by the sum of two exponentials (SSE improvement;CON, 12.02 ± 3.65%; FPI, 15.86 ± 6.30%; see Materialsand Methods). Indeed, similar to the results in response toorthodromic perforant path stimulation, neither the decay timeconstants (Fig. 5C) ( ${tau}$ _decay1; CON, 1.48 ± 0.29 sec; FPI, 1.40 ± 0.28 sec; ${tau}$ _decay2; CON, 7.76 ± 2.89 sec; FPI, 7.69 ± 1.54 sec; n = 12 CON and n = 11 FPI) nor the half-time of recovery (Fig. 5C, inset) (CON: 1.70 ±0.12 sec, n = 15; FPI: 1.38 ± 0.10 sec, n = 11) of theantidromically evoked [K⁺]_o elevation in response to a trainof 10 stimuli were increased in the slices from head-injuredanimals. If anything, there was a slight trend toward a faster(rather than slower) half-time of recovery of the potassiumtransient after injury.
The fortuitous observation that the [K⁺]_o elevation in responseto eight stimuli in the control tissue and five stimuli in the injured tissue was similar (Fig. 5B) provided us with an opportunityto examine differences in the clearance of stimulation-evoked[K⁺]_o transients between control and traumatized tissue withoutthe confounding effects of differences in the amplitude ofevoked [K⁺]_o elevation. The decay time constants of the antidromicallyevoked [K⁺]_o transients of similar amplitude was not increased after head injury ( ${tau}$ _decay1; CON, 1.46 ± 0.19 sec; FPI, 1.63 ± 0.23 sec; ${tau}$ _decay2; CON, 8.36 ± 2.05 sec; FPI, 6.61 ± 0.99 sec). These data confirmed that theclearance of [K⁺]_o was not compromised after 1 week after headinjury and, therefore, was not the cause of the larger post-traumaticincrease in the antidromically evoked [K⁺]_o transient. Additional experiments performed to further examine this issue at differenttime points and locations showed that, similar to our datafrom 1 week described above, the half-time of recovery of theantidromically evoked [K⁺]_o increases was not increased either2 d or 1 month after injury, either in the granule cell layer (Fig. 5D) (half-time of recovery; 2 d after injury: CON, 1.68± 0.13 sec, n = 9; FPI, 1.60 ± 0.11 sec, n =9; 1 month after injury: CON, 1.21 ± 0.16 sec, n = 10;FPI, 1.51 ± 0.11 sec, n = 11) or in the CA3 pyramidalcell layer (half-time of recovery; 2 d after injury: CON, 1.68± 0.17 sec, n = 9; FPI, 1.25 ± 0.12 sec, n =9; 1 month after injury: CON, 1.36 ± 0.31 sec, n = 7;FPI, 1.76 ± 0.19 sec, n = 8). These results demonstratethat the rate of clearance of stimulation-evoked [K⁺]_o increasewas not impaired 2 d, 1 week, or 1 month after head injury.
The fact that the antidromically evoked [K⁺]_o increase in ionotropicglutamate and GABA receptor antagonists was larger in the head-injuredanimals (Fig. 5A,B), despite a lack of decrease in the clearanceof [K⁺]_o, prompted us to examine whether the neuronal firingwas enhanced after trauma in the paradigm used in the above experiments. As shown by whole-cell recordings from granulecells in response to a train of 10 stimuli (Fig. 5A, insets),each antidromic stimulus evoked a single action potential (CONand FPI, four of four cells each), confirming that the actionpotential firing evoked by antidromic stimulation of granulecell axons was not different between injured and control animals.Although the individual granule cells fired the same numberof action potentials, the antidromically evoked populationspikes recorded in the granule cell layer simultaneously withthe antidromically evoked [K⁺]_o transients (in Fig. 5) werelarger after head injury (Fig. 6A,B). In addition to the largeramplitude, there was a post-traumatic decrease in the half-width(width at half-maximal amplitude) of the antidromic population spike (Fig. 6C) (CON: 0.73 ± 0.05 msec, n = 15; FPI:0.58 ± 0.03 msec, n = 11), suggesting a greater synchronyin the granule cell firing after head trauma. In fact, thepopulation spike in CA3 evoked by single-shock stimulationof the Schaffer collaterals (at 6 mA stimulation intensity)was also significantly larger 2 d after injury (data not shown;CON, 1.76 ± 0.30 mV; FPI, 2.99 ± 0.47 mV). Overall,similar to the orthodromically evoked [K⁺]_o increase, the largerantidromically evoked [K⁺]_o transient after FPI also occurredin conjunction with increased neuronal population spike. Althoughit is possible that a postinjury decrease in the extracellularspace could contribute to both the enhanced population responseand the larger [K⁺]_o transient (Jefferys, 1995; Nicholsonet al., 2000), it is evident that the activity of populationsof neurons in control and pathological conditions is not thesame in the above experimental paradigm, possibly as a resultof plastic changes in the neuronal networks (e.g., sproutingof the axons of principal cells after trauma) (McKinney etal., 1997; Santhakumar et al., 2001).

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Figure 6. Hyperexcitable granule cell field responses to antidromic stimulation. A, Examples of population spikes evoked by antidromic stimulation of the granule cells (at 6 mA stimulation intensity) in the same slices as in Figure 5A from an injured animal (FPI) and sham-control animal (CON) are shown. B, Summary data of the antidromic population spike amplitudes during the [K ⁺]_o recordings shown in the top inset in Figure 5B demonstrate an increase in the population spike amplitude 1 week after FPI. C, Summary plot shows that the half-width of the antidromically evoked population spike was decreased after head trauma.

Post-traumatic decrease in granule cell response to [K⁺]_o
Finally, we investigated the possibility that [K⁺]_o transientscould still play a mechanistic role in the postinjury granulecell hyperexcitability even in the absence of impaired bufferingof [K⁺]_o, if the same [K⁺]_o increase evoked a larger depolarizationand more action potential firing in the neurons after headinjury. Brief application (10 msec) of ACSF containing 120 mM potassium through a glass pipette located at a constant distance (50 µm) from the recording electrode in the bath abovethe surface of the slice in the direction of flow of the perfusate,with a constant orientation of the slice, was used to evokegranule cell depolarization and firing. Whole-cell recordingswere obtained from granule cells in ionotropic glutamate andGABA receptor antagonists to prevent polysynaptic activity.Surprisingly, potassium application evoked a smaller depolarization (Fig. 7A,B) (CON: 32.25 ± 4.99 mV, n = 12; FPI: 17.58± 4.66 mV, n = 11) in head-injured animals. Furthermore,potassium application also evoked action potential firing infewer granule cells after head trauma (CON: 70%, n = 10; FPI:21%, n = 14), indicating a post-traumatic decrease in sensitivityto [K⁺]_o elevation. These data show that not only is thereno evidence for impaired buffering of [K⁺]_o, but the responseof granule cells to [K⁺]_o transients is actually decreasedafter head trauma.
Although our main focus was to test the impaired [K⁺]_o bufferinghypothesis of post-traumatic hyperexcitability (D'Ambrosioet al., 1999), an additional interesting point concerns themechanisms that may cause the postinjury decrease in granulecell sensitivity to [K⁺]_o increases described above. What madethe injured granule cells less responsive to [K⁺]_o increases? Previous studies have shown that the resting membrane potential,input resistance, and threshold for action potential generationare not different between granule cells from injured and controlanimals (Santhakumar et al., 2000). In agreement with theseprevious results, steady-state current–voltage (I/V)plots from granule cells in head-injured animals (n = 5 cells)and control animals (n = 5 cells) showed no difference in eitherthe resting membrane potential (data not shown) or the slopeof the I/V plots for negative current steps between +50 pAand -400 pA (Fig. 7C). Additionally, a subset (n = 3 cellseach) of the granule cells that showed stable voltage responsesto current injections between +50 pA and -700 pA also did notreveal a significant difference in the slope of the I/V plotsfrom injured and control animals (Fig. 7C, inset) (note thatif anything, there was a slight trend at very hyper-polarizedpotentials for the granule cells after injury to show lesschange in voltage to a given large current step, i.e., in theopposite direction of what would be expected if the potassiumpermeability were decreased due to fewer or less active potassiumchannels). However, an alternative approach for the identification of the mechanism of post-traumatic decrease in the potassium-evoked depolarization is to block the potassium channels with intracellularQX-314, a nonspecific potassium and sodium channel blocker.Intracellular application of QX-314 has been shown to decreasethe neuronal responses to externally applied potassium (Smirnovet al., 1999). When QX-314 was included in the internal solutionin our experiments, the differences in potassium-evoked membranedepolarization between granule cells from injured and controlanimals were abolished (Fig. 7B, inset) (CON: 21.67 ±8.5 mV, n = 7; FPI: 18.31 ± 7.7 mV, n = 6). Furthermore,the depolarization evoked by potassium application in the controltissue was reduced to a level similar to that of the granulecells from injured animals. The fact that intracellular QX-314inside the recorded neuron could occlude the post-traumaticdecrease in the potassium-evoked depolarization indicates thatthe underlying mechanisms involve differences in the expressionof potassium channels, even if the steady-state I/V plots couldnot reveal such differences. In addition, the lack of a complete block of the potassium-evoked depolarization by intracellularQX-314 in these experiments could be due to various factors,e.g., there may be potassium channels that are not fully blockedby intracellular QX-314.

   Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

This study systematically tested the hypothesis that impaired [K⁺]_o buffering underlies post-traumatic neuronal hyperexcitability(D'Ambrosio et al., 1999). First, we reexamined the resting [K⁺]_o in both the dentate gyrus and CA3 at various time pointsafter injury but found no evidence for an elevated resting [K⁺]_o. Next, we reevaluated the experimental paradigm thatwas proposed to normalize neuronal activity between the controland injured circuits to study deficits in [K⁺]_o regulation and found post-traumatic alterations in the neuronal populationactivity evoked by antidromic stimulation in ionotropic receptorantagonists. Moreover, examination of the rate of clearanceof [K⁺]_o increases evoked either by orthodromic stimulationor after exogenous potassium application did not reveal anypostinjury decrease in [K⁺]_o regulation. In fact, the decreasein potassium-evoked depolarization in neurons from head-injuredanimals suggests a post-traumatic decrease in sensitivity to[K⁺]_o elevation.
[K⁺]_o buffering after head injury
Concussive brain injury causes an immediate increase in theresting [K⁺]_o in vivo that returns to control levels withina few hours (Takahashi et al., 1981; Katayama et al., 1990).In agreement with the rapid recovery of resting [K⁺]_o, theresting membrane potential of granule cells in vitro is similarto controls within hours after in vivo trauma (Ross and Soltesz, 2000; Santhakumar et al., 2000). Our data showed no increasein the resting [K⁺]_o after FPI, in slices in which post-traumatic hyperexcitability in the dentate gyrus was directly verified,despite a recent study indicating that elevated resting [K⁺]_oin hippocampal slices was responsible for the postinjury neuronal hyperexcitability (D'Ambrosio et al., 1999). Furthermore, therewas no increase in the resting [K⁺]_o in either the dentategyrus or CA3, either 2 d or 1 month after trauma. The possiblesources of the discrepancy between the data from D'Ambrosioet al. (1999) and the present study could be that the formerstudy used ACSF containing 4.3 mM potassium and measured baseline[K⁺]_o during low-frequency stimulation (0.05 Hz) at room temperature,whereas we measured the resting [K⁺]_o in the absence of evoked neuronal activity at 36°C in a perfuste containing 2.5 mM potassium, comparable with the [K⁺]_o measured in vivo (Princeet al., 1973; Somjen, 1979; Somjen and Giacchino, 1985; Xiongand Stringer, 1999) and used in previous studies (Rose andRansom, 1996; Xiong and Stringer, 2000; Brickley et al., 2001).In addition, it should be pointed out that a persistent increasein the resting [K⁺]_o in slices is unlikely because the bathsolution would be expected to act as an infinite potassiumsink and remove any post-traumatic, steady-state increase in[K⁺]_o.
We also examined the rate of clearance of the [K⁺]_o elevationevoked by neuronal activity during the decay phase of the [K⁺]_otransient (Xiong and Stringer, 1999). The half-time of recoveryof the [K⁺]_o transient provided a measure of the clearanceof [K⁺]_o that was normalized for the absolute level of the[K⁺]_o increase. The rate of clearance of the [K⁺]_o increaseevoked by either orthodromic or antidromic stimulation wasnot compromised after trauma. Similarly, there was no postinjuryimpairment in the clearance of [K⁺]_o transients after eitherhigh-frequency or single-shock orthodromic stimulation, orafter exogenous potassium application. Overall, our data showthat there is no decrease in the recovery of [K⁺]_o after headinjury at any of the time points examined.
Interestingly, whereas the decay of the single-shock stimulation-evoked [K⁺]_o transient was adequately fit by a single exponential,the larger [K⁺]_o increases, in response to both potassium applicationand to high-frequency, antidromic stimulation, were betterfit by the sum of two exponentials, consistent with the contributionof different mechanisms of [K⁺]_o regulation with increasing [K⁺]_o (Hertz, 1978; Rose and Ransom, 1996). Several processes,including diffusion through extracellular space, spatial bufferingthrough glial K_IR, and active (e.g., via the Na⁺/K⁺ ATPase)and passive potassium uptake, are known to regulate [K⁺]_o (Orkand et al., 1966; Heinemann and Lux, 1975; Ballanyi etal., 1984; Newman et al., 1984; Nicholson, 1995; Walz, 2000).However, the proportion of the [K⁺]_o cleared by each of these processes is not fully known in the normal brain (Walz, 2000; Steinhauser and Seifert, 2002), and their contributions mightvary in pathophysiological states (Onozuka et al., 1987; MacFarlaneand Sontheimer, 1997; Bordey and Sontheimer, 1998; Walz andWuttke, 1999; Schroder et al., 1999; Xiong and Stringer, 2000; Hinterkeuser et al., 2000; Amzica et al., 2002). Nevertheless,although the role of individual regulatory mechanisms in maintaining[K⁺]_o homeostasis might change after brain injury, our resultsshow that the buffering of stimulation-evoked [K⁺]_o elevationis not decreased, indicating that impaired clearance of [K⁺]_odoes not underlie post-traumatic dentate hyperexcitability.
Changes in granule cell excitability during antidromic stimulationand exogenous K⁺ application after head trauma
The present study examined the validity of antidromic activationof neurons in the presence of glutamate receptor antagonists (D'Ambrosio et al., 1999), a paradigm that was proposed tobe useful to evaluate the [K⁺]_o regulation without the confoundingeffects of postinjury increases in neuronal excitability. Ourdata showed that granule cells responded with a single actionpotential to each antidromic stimulus under these conditions.However, the amplitude of the antidromic population spike waslarger after trauma, suggesting that more neurons were firingwith greater synchrony after head injury. It is likely thatthe presence of post-traumatic mossy fiber sprouting (Santhakumaret al., 2001) contributes to the activation of a greater populationof granule cells in response to antidromic stimulation, resultingin a larger antidromic population spike. In addition, it ispossible that a decrease in the extracellular volume fractionand tissue conductivity (Jefferys, 1995) contribute to theincrease in the amplitude of the population spike and [K⁺]_oelevation evoked either by orthodromic or antidromic stimulationof granule cells after head trauma. However, the presence ofincreased stimulus-evoked neuronal activity and hilar cell loss after head injury confounds the meaningful comparison of thealterations in extracellular volume fraction during neuronalactivity, between control and injured animals. Although thefactors underlying the enhanced antidromically evoked populationresponse after head trauma are not known, our results show that the postinjury alteration in the neuronal population activityand not a decrease in the clearance of [K⁺]_o underlies the enhanced [K⁺]_o elevation in an antidromic stimulation-basedparadigm.
A mechanism by which stimulation-evoked [K⁺]_o elevation couldtrigger post-traumatic hyperexcitability, even in the absence of decreased potassium buffering, is whether [K⁺]_o increasescaused greater firing in the granule cells from head-injured animals. Contrary to the above idea, our results show that granulecells responded to potassium application with smaller depolarizationand less action potential firing after FPI. Although the steady-stateI/V curves from granule cells in injured and control animalswere similar, the potassium-evoked depolarization of granulecells from control animals was decreased to postinjury levelswhen potassium channels were blocked by intracellular QX-314inside the recorded neuron. These data are consistent witha post-traumatic decrease in the potassium permeability, notrevealed by the I/V plots, contributing to the smaller amplitudeof the potassium-evoked depolarization in granule cell afterhead trauma. Although it is possible that the enhanced [K⁺]_otransients during neuronal activity may contribute to neuronalhyperexcitability by increasing the presynaptic axon terminalexcitability (Noebels and Prince, 1978; Stasheff et al., 1993),these results show that granule cells from head-injured animalsare hypo-excitable in response to [K⁺]_o increases, indicatingthat stimulation-evoked [K⁺]_o transients cannot directly underliegranule cell hyperexcitability.
Post-traumatic increase in stimulation-evoked [K⁺]_o transient:the cause or result of neuronal hyperexcitability?
In several experiments, we examined whether increased neuronalfiring could account for the larger amplitude of the stimulation-evoked [K⁺]_o transients after injury. The response time of the ISMEwas evaluated to determine whether the electrodes could be usedto study the time course of the early phase of [K⁺]_o elevation evoked by single-shock stimulation [see Fig. 8; also see Appendix (available at www.jneurosci.org)]. The electrodes could detect[K⁺]_o increases within a few milliseconds, consistent withprevious studies (Prince et al., 1973; Lux and Neher, 1973; Moody et al., 1974; Amzica et al., 2002), and revealed a fasterrise and a shorter latency to orthodromically evoked [K⁺]_otransients after injury. Although there was no post-traumaticincrease in the [K⁺]_o transient evoked by afferent stimulationin postsynaptic receptors antagonists, the orthodromicallyevoked granule cell population spike occurred earlier after trauma, suggesting that the shorter latency to neuronal responsecould contribute to the faster postinjury [K⁺]_o increase. Consistent with the shorter latency to the evoked populationspike, whole-cell recordings from granule cells demonstratedan earlier onset of firing in response to perforant path stimulationafter head trauma. In addition to the faster onset, the greaternumber of postsynaptic action potentials fired in responseto perforant path stimulation (Santhakumar et al., 2000) mightcontribute to the larger amplitude, shorter latency, and fasterrise of the orthodromically evoked [K⁺]_o elevation. In addition, the post-traumatic hyperexcitability of certain nonprincipalcells in the dentate gyrus, e.g., the mossy cells (Santhakumaret al., 2000) or GABAergic cells (Ross and Soltesz, 2000;Santhakumar et al., 2001), could also contribute to the augmentationof the evoked [K⁺]_o increase. Overall, in agreement with therole for neuronal activity in postinjury epileptogenesis (Graberand Prince, 1999), our results underscore the role for theincrease in neuronal activity, rather than an impaired [K⁺]_obuffering, as the primary mechanism for the enhanced risk forseizures after head injury.

   Footnotes

Received Feb. 19, 2003; revised May. 6, 2003; accepted May. 9, 2003.
This work was supported by National Institutes of Health GrantNS35915 (I.S.). We thank Dr. Bala Chidambaram and R. Zhu forexpert technical assistance.
Correspondence should be addressed to Dr. Vijayalakshmi Santhakumar, Department of Anatomy and Neurobiology, University of California,Irvine, CA 92697-1280. E-mail: vsanthak{at}uci.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235865-12$15.00/0

   References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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