Sodium Influx Blockade and Hypoxic Damage to CA1 Pyramidal Neurons in Rat Hippocampal Slices

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Sodium Influx Blockade and Hypoxic Damage to CA1 Pyramidal Neurons in Rat Hippocampal Slices

K. M. Raley-Susman,¹ I. S. Kass,²^,³ J. E. Cottrell,² R. B. Newman,¹ G. Chambers,² and J. Wang²

¹Department of Biology, Vassar College, Poughkeepsie 12604; and ²Department of Anesthesiology and ³Department of Physiology and Pharmacology, State University of New York Health Science Center, Brooklyn, New York 11203

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Raley-Susman, K. M., I. S. Kass, J. E. Cottrell, R. B. Newman, G. Chambers, and J. Wang. Sodium Influx Blockade and Hypoxic Damage to CA1 Pyramidal Neurons in Rat Hippocampal Slices. J. Neurophysiol. 86: 2715-2726, 2001. We studied the effects of lidocaine and tetrodotoxin (TTX) on hypoxic changes in CA1 pyramidal neurons to examine the ionicbasis of neuronal damage. Lidocaine (10 and 100 µM) and TTX (6and 63 nM) delayed and attenuated the hypoxic depolarization andimproved recovery of the resting and action potentials after 10min of hypoxia. Lidocaine (10 and 100 µM) and TTX (63 nM) reducedthe number of morphologically damaged CA1 cells and improved proteinsynthesis measured after 10 min hypoxia. Lidocaine (10 µM) attenuatedthe increase in intracellular sodium (181 vs. 218%) and the depolarization( $-$ 21 vs. $-$ 1 mV) during hypoxia but did not significantly attenuatethe changes in ATP, potassium, or calcium measured at 10 min ofhypoxia. Lidocaine (100 µM) attenuated the changes in membranepotential, sodium, potassium, ATP, and calcium during hypoxia.TTX (63 nM) attenuated the changes in membrane potential ( $-$ 36vs. $-$ 1 mV), sodium (179 vs. 226%), potassium (78 vs. 50%), andATP (24 vs. 11%) but did not significantly attenuate the increasein calcium during hypoxia. These data indicate that the primaryblockade of sodium channels can secondarily alter other cellularparameters. The hypoxic depolarization and the increase in intracellularsodium appear to be important triggers of hypoxic damage independentof their effect on cytosolic calcium; a treatment that selectivelyblocked sodium influx (lidocaine 10 µM) improved recovery. Ourdata indicate that selective blockade of sodium channels witha low concentration of lidocaine or TTX improves recovery afterhypoxia by attenuating the rise in cellular sodium and the hypoxicdepolarization. This blockade improves the resting and actionpotentials, histologic state, and protein synthesis of CA1 pyramidalneurons after 10 min of hypoxia to rat hippocampal slices. A higherconcentration of lidocaine, which also improved ATP, potassium,and calcium concentrations during hypoxia was more potent. Inconclusion, the depolarization and increased sodium concentrationduring hypoxia account for a portion of the neuronal damage afterhypoxia independent of changes incalcium.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Ischemia and hypoxia of the brain lead to irreversible neuronal damage and cause death and disability. In this paper we investigatethe effect of interrupting sodium influx, one component of theischemic and hypoxiccascade.

It is known that during hypoxia and ischemia there is a depolarization of the neurons that is associated with a change intheir intracellular ionic composition; altering the ionic environmentof these neurons attenuates this change (Hansen 1985; Tanaka etal. 1997). Sodium influx increases early during hypoxia and appearsto be an important component of the rapid depolarization (Hansen1985; Tanaka et al. 1997). Sodium is an ion that is central tocellular homeostasis; its gradient across the cell membrane isused as an energy source to transport calcium, glutamate, andhydrogen (Choi 1992; Siesjo and Siesjo 1996). These componentsare thought to be important determinants or triggers of neuronaldamage. Glutamate-induced excitotoxicity has been implicated asan important trigger of hypoxic damage (Choi 1992). High cytosolicsodium concentrations can reverse the glutamate transporter, causerelease of glutamate, and enhance excitotoxicity (Roettger andLipton 1996). Much evidence exists to establish the importanceof calcium as a trigger of hypoxic damage (Kass and Lipton 1982,1986; Lipton 1999; Siesjo 1991); there is little evidence of sodium'srole during hypoxia independent from its effect on calcium. Thispaper examines whether reducing the intracellular sodium accumulationand the depolarization during hypoxia without significantly alteringcytosolic calcium can improve recovery afterhypoxia.

It has been established that blockade of sodium channels can reduce hypoxic or ischemic damage (Astrup et al. 1981; Boeninget al. 1989; Lucas et al. 1989; Stys et al. 1992; Weber and Taylor1994). Lidocaine and tetrodotoxin block sodium channels; lidocaineat high concentrations can also block potassium efflux and othercellular processes (Astrup et al. 1981; Strichartz and Ritchie1987). Tetrodotoxin is highly specific for the sodium channel.The low concentration of lidocaine used in our study is similarto an antiarrhythmic dose used clinically and does not disruptneuronal activity (Fried et al. 1995; Lucas et al. 1989; Styset al. 1992; Weber and Taylor 1994). There is evidence that lidocainecan improve recovery both in animals in vivo and clinically (Leiet al. 2001; Liu et al. 1997; Mitchell et al. 1999; Shokunbi etal. 1990). We have used intracellular recording techniques, histologicalanalysis, measurement of protein synthesis, and cytosolic calciumconcentration measurements to improve our understanding of howthe blockade of sodium influx during hypoxia improvesrecovery.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Slice preparation

The experiments were approved by the Institutional Animal Care and Use Committee and conform to National Institutes of Healthguidelines. Many of the techniques used in this paper have beenreported by us before and will be described briefly (Fried etal. 1995; Kass et al. 1992; Raley-Susman and Lipton 1990; Raley-Susmanet al. 1997; Wang et al. 1999, 2000). For each experiment an adultSprague- Dawley rat (110-120 days old) was anesthetized with 2%isoflurane until it lost its righting reflex and was unresponsiveto touch (Zhu et al. 1997). The rat was then decapitated, itsbrain removed and placed in ice-cold (2-4°C) artificial cerebrospinalfluid (ACSF). The hippocampus was dissected from the brain andsliced transversely. ACSF contained (in mM) 126 NaCl, 3 KCl, 1.4KH₂PO₄, 26 NaHCO_3, 4 glucose, 1.3 MgSO₄, and 1.4 CaCl₂, with pH7.4, and was equilibrated with 95% O₂-5% CO₂. Hypoxia was generatedby switching to ACSF preequilibrated with 95% N₂-5% CO₂. Duringhypoxia the slice is continuously superfused with ACSF containing4 mM glucose. This is a less severe insult than that used in manyother slice studies of in vitro ischemia in which the ACSF isswitched to 0 glucose during the hypoxia. Both models wash potentiallytoxic metabolites from the slice during the hypoxic/ischemic period.Unless indicated in the text, the duration of hypoxia is 10 min.In the drug-treated groups, slices were exposed to drug 10 minbefore and during 10 min of hypoxia. Two concentrations of lidocaine(10 and 100 µM) and tetrodotoxin (6 and 63 nM) were examined.The slices were maintained at 37°C during theexperiments.

Electrophysiology

For the electrophysiology experiments, 400-µm slices were prepared with a vibratome, incubated at room temperature, and thenplaced in a tissue chamber (Fine Science Tools) at 37°C. Multipleslices from the same animal were transferred to the tissue chamberserially to minimize the number of animals used. The slices weresubmerged 1 mm below the ACSF surface in the tissue chamber andsuperfused at a rate of 3 ml/min. Intracellular recordings ofCA1 pyramidal neurons were made with glass micropipettes filledwith 4 M KAc. The resistance of the electrodes ranged from 70to 120 M $Omega$ . A bipolar stimulating electrode was placed in the Schaffercollateral pathway before impaling the CA1 neuron. Only neuronswith stable resting potentials of at least $-$ 55 mV for 15 min withhigh-amplitude, short-duration action potentials that showed spikefrequency accommodation and were activated by short-latency Schaffercollateral stimulation were examined. These parameters are characteristicof CA1 pyramidal cells, and our recordings were typically stablefor over 1 h. Analog signals were recorded with an AxoClamp 2Bamplifier and an IBM-compatiblecomputer.

Protein synthesis and morphology

In the experiments that examined protein synthesis and morphology, slices were exposed to either lidocaine or TTX 15 min before,during, and 15 min after 10 min of hypoxia. Forty-five minutesafter the end of the 10-min hypoxia, 4.5 µCi/ml [³H]leucine was added to each beaker, and the slices were allowedto incorporate the label into protein for an additional 75 minafter the insult. Slices were washed in ice-cold buffer for 3min to remove extracellular unincorporated label and were fixedovernight in 4% paraformaldehyde in 0.1 M phosphate buffer at4°C. [³H]leucine incorporated into protein, but not free unincorporatedintracellular leucine, is retained by the tissue (Raley-Susmanand Lipton 1990). Based on our previous measurements in responseto anoxia/aglycemia, changes in incorporation reflect changesin protein synthesis, not changes in the specific activity ofthe precursor pool or in the pool of free unlabeled leucine (Raley-Susmanand Barnes 1998; Raley-Susman and Lipton 1990). Slices were dehydratedand embedded in methyl acrylate. Five-micrometer sections weremounted on coated slides and dipped in NTB2 emulsion (Kodak) forautoradiographic assessment of protein synthesis. Autoradiographswere digitized and analyzed as described previously (Wang et al.1999), where silver grain density is proportional to the amountof radioactivity incorporated into protein. Densities from experimentalgroups were compared with densities of normoxic control sectionstreated identically on the sameslides.

Morphological assessment was performed on adjacent 20-µm tissue sections using light microscopy as described by us previously(Wang et al. 1999). In brief, we scored the histologic class ofall neurons in the CA1 pyramidal layer of a tissue section fromeach slice. Healthy neurons (class A) had intact cell boundaries,a clear uniform nucleus and clear cytoplasm. Unhealthy neurons(class C) were either indistinct, lacking a clear cell boundary,with a small darkened nucleus, or darkened, shrunken cells. Therewere a number of neurons in each slice that exhibited an intermediatedamaged morphology, class B, suggestive of a progression of damage.For simplicity, we focused our analysis on the class A and classC neurons. The percentage of the intermediate neurons (class B)did not change between normoxic and hypoxic conditions (data notshown). We examined the morphology of neurons 2 h after the hypoxicinsult to correspond temporally with the protein synthesis measurement.This time point is after many reversible changes have recoveredtoward normoxic levels, thus at a time preceding overt celldeath.

ATP, Na, and K measurements

Slices (500 µm) were prepared using a manual tissue slicer and mounted on nylon mesh attached to a Plexiglas grid. The useof a manual tissue slicer allowed a greater number of slices tobe obtained from each animal and substantially reduced the numberof animals required for these experiments. The grids were thenplaced in beakers containing ACSF. Slices from the same animalwere distributed to beakers subjected to either control or experimentaltreatments. The slices were incubated at room temperature for45 min, and then the temperature was increased to 37°C and maintainedat that temperature for the rest of the experiment. The sliceswere subjected to hypoxia 75 min after shifting to 37°C. The ACSFin the beaker was aerated with 95% O₂-5% CO₂; to generate hypoxiathe ACSF in the beaker was aerated with 95% N₂-5% CO₂. Sodium,potassium, and ATP levels in tissue from the CA1 region were measuredbefore and duringhypoxia.

ATP concentrations were measured in the CA 1 regions from slices frozen in liquid nitrogen and lyophilized to complete dryness(4.5 h). The CA1 regions were microdissected and weighed, andthe ATP was extracted in perchloric acid frozen on dry ice (Kass1986). The neutralized extract was assayed in a photometer usingthe luciferin-luciferase assay (Lust et al. 1981).

Sodium and potassium were measured using a flame photometer. At each time point, slices were placed in agitated ice-cold (4°C)isotonic sucrose for 10 min to wash ions from the extracellularspace (Kass et al. 1992). The CA1 regions of the slices were rapidlymicrodissected, placed on preweighed aluminum foil boats, driedat 85°C for 48 h, and weighed. Each boat, which contained thepooled CA1 regions of all the slices from a single beaker, wasplaced in a 0.5-ml microcentrifuge tube. Dilute nitric acid (0.1N) was added to the tubes that were then shaken for 16 h to extractions from the tissue. The tubes were centrifuged at 13 K for 1min, and the supernatant was assayed in a flame photometer (Friedet al. 1995).

To measure cellular sodium accurately, the sodium in the extracellular space of the slice needs to be washed out; however,there is a small loss of ions from the intracellular space whilewashing out the extracellular space of the slice. We have optimizedthe wash out conditions for sodium (Kass et al. 1992) such thatthere is minimal loss of cellular sodium. There is a sharp differencein slope of the sodium wash out indicating two major pools: aninitial fast component is indicative of the extracellular pooland a much slower component is indicative of wash out from theintracellular space. At 10 min of wash out in ice-cold isotonicsucrose, the slope of the sodium in the fast component extrapolatedto 0 while there was only a minimal effect on sodium from theslow component (the intracellular pool) (Kass et al. 1992). Potassiumwash out did not separate neatly into two very different slopes,and 10 min in isotonic sucrose caused a relatively greater lossof potassium during wash out. One interpretation of this is thatthere is enhanced cellular permeability to potassium replenishingthe extracellular space leading to a reduced fast component (Kasset al. 1992). Therefore the potassium concentrations measuredare lower than their true level. We are more interested in thesodium levels and that is why we optimized the technique to measuresodium. All the tissue in our study was treated identically, andrelative changes in the amount of sodium and potassium arecompared.

Calcium imaging

Slices for Ca imaging were sectioned to a thickness of 300 µm on a vibratome. These thinner slices improved the visualizationof tissue in the microscope and dye loading. Slices were incubatedin oxygenated ACSF for at least 2 h before dye loading. Two sliceswere then placed in a small beaker with 6 ml ACSF containing 9µM Fura 2 AM (Molecular Probes; Eugene, OR), 0.01% pluronic acidand 50 µl DMSO for 45 min, washed in fresh ACSF and incubatedfor an additional 45 min to allow the AM moiety to hydrolyze fromthe Fura-2 (Wang et al. 1999, 2000). The slices were maintainedat 33°C from the initial incubation until they were placed ina tissue chamber on the microscope stage; maintenance at thistemperature improved dye loading. The slices were maintained at37°C in the tissue chamber on the microscope stage throughoutthe experiment. An InCyt Im2 dual wave length imaging system witha low light level charge-coupled device (CCD) camera was used(Intracellular Imaging, Cincinnati, OH). A long working distanceNikon Plan Fluor ×20 ultraviolet objective (n.a. 0.5) and a NikonTMS inverted microscope were attached to a filter changer (340-and 380-nm filters), a 300-W Xenon light source and the CCD camerafor image acquisition. The calcium concentrations were measuredfrom a region that included the CA1 stratum pyramidale and theproximal third of the stratum oriens and the stratumradiatum.

We used Ca²⁺ buffers in solution and Fura-2 salt (Molecular Probes) to calibrate the imaging system for Ca concentration. Allvalues represent Ca concentrations corrected for background fluorescencein time-matched, unlabeled (no Fura2) slices subjected to hypoxia(Wang et al. 2000). This was done to correct for the increasein background fluorescence due to the increase in NADH levelsduring hypoxia (Brooke et al. 1996).

Statistics

A $chi$ ² test was used to analyze recovery in the electrophysiological experiments. To statistically analyze the morphologic changes,data were transformed using an arcsine transformation of the squareroot of each value (Motulsky 1999). These transformed data thenfit a normal distribution and were analyzed using an ANOVA followedby the Newman-Keuls test for multiple comparisons. The proteinsynthesis, ATP, sodium, potassium, and calcium data were analyzedusing an ANOVA followed by the Newman-Keuls multiple comparisontest (Prism, GraphPad Software, San Diego, CA). P < 0.05 was consideredsignificant for allanalyses.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Membrane potential changes

During hypoxia there is an initial hyperpolarization followed by a slow then a rapid depolarization (Fig. 1A). In untreatedhippocampal slices, 10% of the CA1 pyramidal cells recovered theirnormal resting potential and their ability to generate actionpotentials after 10 min of hypoxia. A low concentration of lidocaine(10 µM), which did not alter the excitability of the neurons beforehypoxia, significantly improved recovery of membrane potentialsand excitability after hypoxia; 67% of the CA1 pyramidal neuronsrecovered (Fig. 1B). A higher concentration of lidocaine (100µM) also significantly improved recovery when compared with untreatedslices (80% of the neurons recovered); there was no significantdifference in recovery between the 10- and 100-µM lidocaine groupsafter 10 min of hypoxia. If the hypoxic period was extended to15 min, then 100 µM, but not 10 µM lidocaine, significantly improvedrecovery (Fig. 2B). Thus the higher concentration is more potentagainst the effects of prolonged hypoxia.

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Fig. 1. Effect of lidocaine on recovery of membrane and action potentials after 10 min hypoxia. A: the membrane potentials (mean ± SE) of CA1 pyramidal cells during hypoxia with 0, 10, and 100 µM lidocaine. Lidocaine significantly delays the onset of the rapid depolarization and the level of depolarization at 10 min hypoxia. B: percent of CA1 pyramidal neurons that recover their resting and action potentials after 10 min hypoxia. In slices treated with lidocaine 10 µM (n = 21) and 100 µM (n = 10), there was significantly better recovery compared with untreated slices (n = 21) after 10 min hypoxia (*P < 0.01, $chi$ ² test). C: an example of intracellular electrophysiologic recordings of an individual experiment from each treatment group. The 1st trace in each set is the response recorded from a CA1 pyramidal cell after stimulation of the Schaffer collateral pathway; the 2nd and 3rd trace in each set is during 100- and 200-pA current injection through the recording electrode. Sets of traces are shown in each treatment group: before drug, 10 min after drug application before hypoxia, during 10 min hypoxia with drug, and 60 min after reoxygenation and drug wash out. The excitability of neurons before hypoxia was not altered by 10 µM lidocaine. The neurons treated with 10 and 100 µM lidocaine recovered their ability to be excited; however, the threshold to evoke action potentials was increased, and their response to stimulation was not as robust after hypoxia.

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Fig. 2. Effect of lidocaine on recovery of membrane and action potentials after 15 min hypoxia. A: the membrane potentials (mean ± SE) of CA1 pyramidal cells during hypoxia with 0, 10, and 100 µM lidocaine. Lidocaine (100 µM but not 10 µM) significantly reduces the level of depolarization at 15 min hypoxia. B: percent of CA1 pyramidal neurons that recover their resting and action potentials after 15 min hypoxia. In slices treated with 100 µM lidocaine (n = 8), there was significantly better recovery compared with untreated slices (n = 10) after 10 min hypoxia (*P < 0.01, $chi$ ² test).

The slow depolarization during hypoxia is prolonged and attenuated by 10 µM lidocaine such that the neuron does not becomecompletely depolarized after 10 min of hypoxia (Fig. 1A). Onehundred micromolar lidocaine further reduced this depolarization.At 15 min of hypoxia, the 10-µM lidocaine group was completelydepolarized and did not recover while the 100-µM lidocaine groupwas depolarized to the same level as the 10 µM after 10 min ofhypoxia (Fig. 2A). Thus it seems that complete depolarizationduring hypoxia leads to the loss of membrane potential recoveryafterhypoxia.

A high concentration of lidocaine (100 µM) markedly decreases excitability to both orthodromic activation and intracellularcurrent injection before hypoxia; 10 µM lidocaine has no effecton excitability (Fig. 1C). After 10 min of hypoxia, CA1 cellsfrom both the 10- and 100-µM lidocaine groups recover their restingand actionpotentials.

The mean time after hypoxia for recovery to 50% of the resting potential with 10 µM lidocaine was 2.95 ± 0.70 (SE) min, while100 µM lidocaine shortened this time to 1.17 ± 0.25 min; thesevalues were not significantlydifferent.

The threshold for action potential generation with current injection was elevated in both the 10- and the 100-µM lidocainegroups 60 min after hypoxia (15 and 0% of the neurons generatedaction potentials, respectively, at 100 pA; 54 and 67% at 200pA; 100 and 100% at 300 pA) compared with the threshold beforehypoxia and drug addition (82% at 100 pA). This indicates a reductionof excitability even though action potential generation is preserved.There was no significant difference between the two lidocaineconcentrations.

Lidocaine has actions other than blocking sodium channels on the cell membrane; we therefore examined the effect of tetrodotoxin(TTX), a drug that selectively blocks certain sodium channels.Any effects on other ions or cellular processes would thereforebe secondary to the blockade of sodiuminflux.

The effect of TTX on the membrane potential changes during hypoxia was similar to that of lidocaine. A low concentration ofTTX (6 nM) prolonged and attenuated the slow depolarization anddelayed the onset of the rapid depolarization (Fig. 3A). A higherconcentration (63 nM) further prolonged the slow depolarizationand blocked the rapid depolarization (Fig. 3A).

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Fig. 3. Effect of tetrodotoxin (TTX) on recovery of membrane and action potentials after 10 min hypoxia. A: membrane potentials (mean ± SE) of CA1 pyramidal cells during hypoxia with 0, 6, and 63 nM TTX. TTX (6 and 63 nM) significantly delays the onset of the rapid depolarization and the level of depolarization at 10 min hypoxia. B: percent of CA1 pyramidal neurons that recover their resting and action potentials after 10 min hypoxia. In slices treated with TTX 6 nM (n = 26) and 63 nM (n = 15), there was significantly better recovery compared with untreated slices (n = 28) after 10 min hypoxia (⁺P < 0.05; *P < 0.01, $chi$ ² test).

The mean time after hypoxia for recovery to 50% of the resting potential with 6 nM TTX was 3.88 ± 1.44 min, 60 nM TTX shortenedthis time to 1.10 ± 0.20 min, these values were significantlydifferent.

Both concentrations of TTX examined (6 and 63 nM) improved the recovery of the membrane potential and the ability of neuronsto generate action potentials after hypoxia (Fig. 3B). In untreatedslices, no cells recovered after 10 min of hypoxia; 31% of theCA1 pyramidal cells recover if the slices were treated with 6nM TTX, while 73% recovered in slices treated with 63 nMTTX.

Morphology

Two hours after 10 min hypoxia, there is distinct and significant morphological damage (class C cells; see METHODS for a description).We assessed the percentage of CA1 neurons in each slice that exhibitedthis damaged morphology and the corresponding percentage of healthycells (class A cells). Untreated slices showed a substantial lossin the percentage of class A cells in the CA1 region, with a correspondingincrease in class C cells (Fig. 4A). Ten micromolar lidocainesignificantly reduced the percentage of damaged CA1 pyramidalcells 2 h after 10 min of hypoxia (47 vs. 78% in untreated hypoxicslices). One hundred micromolar lidocaine had a similar effecton the morphology (51% damaged cells); there was no significantdifference between the morphology with the two concentrationsof lidocaine.

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Fig. 4. Effect of lidocaine and tetrodotoxin on morphology of CA1 pyramidal neurons after 10 min of hypoxia. Data are the percentage of cells in the CA1 pyramidal cell layer that show either healthy (class A) or damaged (class C) morphology (see METHODS for criteria). All cells in the CA1 cell layer are counted; intermediate morphology cells (class B) are not shown. Data are the means ± SE. All values are compared with the hypoxic untreated value for a particular morphologic class. Statistics were done with transformed data (see METHODS) to assure a normal distribution (*P < 0.01, vs. untreated hypoxic tissue; Newman-Keuls test). A: both 10 µM lidocaine (n = 19) and 100 µM lidocaine (n = 19) significantly increased the number of class A cells and decreased the number of class C cell compared with untreated hypoxia (n = 23). B: 63 nM (n = 18) but not 6 nM (n = 17) TTX significantly increased the number of class A cells and decreased the number of class C cells compared with untreated hypoxia (n = 20).

TTX (63 nM) significantly improved the histology of hypoxic neurons following 10 min hypoxia (Fig. 4B). In untreated slices70% of the CA1 pyramidal neurons appeared damaged (class C cells);this compares with 40% damaged cells from slices treated with63 nM TTX. Six nanomolar TTX did not significantly reduce thepercentage of damaged neurons after 10 min hypoxia (63%).

Protein synthesis

There was dramatic and persistent inhibition of new protein synthesis in the CA1 neurons 2 h after 10 min hypoxia, to 17.3%of normoxic levels (Fig. 5A). Ten micromolar lidocaine significantlyattenuated the inhibition of protein synthesis (to 42% of normoxiclevels), and 100 µM lidocaine preserved protein synthesis to aneven greater degree (67% of normoxic levels). One hundred micromolarlidocaine-treated hypoxic slices had significantly more new proteinsynthesis than 10 µM lidocaine-treated hypoxic slices. Thus whileboth concentrations of lidocaine improved the recovery of proteinsynthesis, the 100-µM concentration was more effective.

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Fig. 5. Effect of lidocaine and tetrodotoxin on protein synthesis in CA1 pyramidal cell layer after 10 min of hypoxia. Protein synthesis was measured as incorporation of ³H-leucine into protein; values (means ± SE) are the average silver grain density expressed as a percentage of CA1 pyramidal cell layer (⁺P < 0.05, *P < 0.01, vs. untreated hypoxic tissue; Newman-Keuls test). A: both 10 µM lidocaine (n = 26) and 100 µM lidocaine (n = 21) had significantly increased protein synthesis compared with untreated hypoxia (n = 23). B: 63 nM (n = 18) but not 6 nM (n = 17) TTX significantly increased protein synthesis compared with untreated hypoxia (n = 20).

In the TTX study, hypoxia caused an inhibition of new protein synthesis to 21.9% of normoxic levels when measured 2 h afterthe insult (Fig. 5B). Six nanomolar TTX did not significantlyattenuate this inhibition (levels were 44% of normoxic proteinsynthesis rates). However, 63 nM TTX significantly improved proteinsynthesis rates after hypoxia to 73% of normoxiclevels.

ATP concentrations

ATP fell to 10% of its normoxic concentration during 10 min of hypoxia; this fall was attenuated to only 22% by 100 µM lidocaine(Fig. 6A). Ten micromolar lidocaine did not significantly alterthe ATP depletion during 10 min of hypoxia; it fell to 15% ofits normoxic concentration.

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Fig. 6. Effect of lidocaine and tetrodotoxin on the ATP concentration in the CA1 pyramidal cell layer at 10 min of hypoxia. Values are the means ± SE (*P < 0.01, vs. untreated hypoxic tissue; Newman-Keuls test). A: 100 µM lidocaine (n = 21), but not 10 µM lidocaine (n = 18), significantly attenuated the fall in ATP (nM/mg dry weight) compared with untreated tissue (n = 24) during hypoxia. B: 63 nM TTX (n = 23), but not 6 nM TTX (n = 25), significantly attenuated the fall in ATP (nM/mg dry weight) compared with untreated tissue (n = 24) during hypoxia.

The fall in ATP during hypoxia was significantly attenuated by 63 nM but not 6 nM TTX (Fig. 6B). ATP fell to 11 and 24% ofits normoxic concentration after 10 min hypoxia with 6 and 63nM TTX,respectively.

Sodium and potassium concentrations

During hypoxia, ATP concentrations were reduced; this should inhibit the Na/K pump and cause sodium to increase dramatically.Sodium increased to 218% of its normal concentration after 10min of hypoxia (Fig. 7A). A low concentration of lidocaine (10µM) significantly attenuated the increase in sodium during hypoxia(to 181% of its concentration with normal oxygen); a higher concentrationof lidocaine (100 µM) further attenuated this increase (155%).Lidocaine significantly reduced the hypoxic sodium influx duringhypoxia; 100 µM was significantly more effective than 10 µM.

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Fig. 7. Effect of lidocaine and tetrodotoxin on the sodium concentration in the CA1 pyramidal cell layer at 10 min of hypoxia. Values are the means ± SE (*P < 0.01, vs. untreated hypoxic tissue; Newman-Keuls test). A: lidocaine (100 and 10 µM), significantly attenuated the rise in sodium (nM/mg dry weight) compared with untreated tissue during hypoxia (n = 6 for all groups). B: 63 nM TTX, but not 6 nM TTX, significantly attenuated the rise in sodium (nM/mg dry weight) compared with untreated tissue during hypoxia (n = 6 for all groups).

The sodium concentration increased to only 179% of its normoxic concentration in slices treated with 63 nM TTX (Fig. 7B).This was significantly attenuated compared with untreated hypoxictissue (226%). There was a small, but not significant, attenuationin the rise in sodium with 6 nM TTX; it rose to 207% of its normoxicconcentration.

There was a decrease in intracellular potassium to 43% of its normal concentration at 10 min of hypoxia; 10 µM lidocaine didnot significantly attenuate the fall in potassium during hypoxia(51% of normoxic concentration) (Fig. 8A). The high concentrationof lidocaine (100 µM) significantly attenuated the fall in intracellularpotassium; potassium fell to only 71%. Thus there is an importantdifference between 10 µM lidocaine's effect on potassium and sodium;the low concentration appears to be selective for sodium.

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Fig. 8. Effect of lidocaine and tetrodotoxin on the potassium concentration in the CA1 pyramidal cell layer at 10 min of hypoxia. Values are the means ± SE (*P < 0.01, vs. untreated hypoxic tissue; Newman-Keuls test). A: 100 µM lidocaine, but not 10 µM lidocaine, significantly attenuated the fall in potassium (nM/mg dry weight) compared with untreated tissue during hypoxia (n = 6 for all groups). B: 63 nM TTX, but not 6 nM TTX, significantly attenuated the fall in potassium (nM/mg dry weight) compared with untreated tissue during hypoxia (n = 6 for all groups).

The higher concentration of TTX (63 nM) significantly attenuated the fall in potassium to only 78% (Fig. 8B). The lower concentrationof TTX (6 nM) had no effect on potassium levels duringhypoxia.

Calcium concentrations

Increased intracellular calcium concentrations have been implicated as a trigger of hypoxic neuronal damage. During 10 minof hypoxia, calcium increased to 241% of its concentration duringnormal oxygenation (Fig. 9A). Ten micromolar lidocaine did notsignificantly attenuate this increase (232%), but 100 µM lidocaineblocked the increase in calcium during hypoxia (128% of its normoxicconcentration).

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Fig. 9. Effect of lidocaine and tetrodotoxin on cytosolic calcium concentrations in the CA1 pyramidal cell layer. Values are the means ± SE. A: cytosolic calcium significantly increased in the untreated (n = 16) and the 10-µM lidocaine (n = 12) groups at 10 min of hypoxia compared with its concentration before hypoxia in that group (P < 0.01, t-test); 100 µM lidocaine (n = 12), but not 10 µM lidocaine (n = 12), significantly attenuated the rise in calcium during hypoxia compared with untreated tissue (n = 16; P < 0.01; Newman-Keuls test). B: cytosolic calcium significantly increased in the untreated (n = 10), the 6-nM TTX (n = 8) and the 63-nM TTX groups at 10 min of hypoxia compared with its concentration before hypoxia in that group (P < 0.01, t-test); TTX (6 or 63 nM) did not significantly attenuate the rise in cytosolic calcium during hypoxia.

The increase in calcium during hypoxia with 63 nM and 6.3 nM TTX was to 186 and 225% of its normoxic concentration, respectively;the calcium concentration at the end of 10 min of hypoxia afterthe application of these TTX concentrations was not significantlydifferent from untreated tissue (Fig. 9B). Thus 63 nM TTX didnot block the change in cytosolic calcium even though it improvedthe recovery of physiologic properties and protein synthesis after10 min ofhypoxia.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We have examined the mechanisms by which blocking sodium channels attenuates hypoxic damage. Both TTX and lidocaine were examinedsince lidocaine has other actions aside from its ability to blocksodium channels (Astrup et al. 1981; Das and Misra 1992). We foundthat concentrations of lidocaine and TTX that attenuated the increasein sodium concentrations and reduced the depolarization duringhypoxia, but did not significantly attenuate the rise in cytosoliccalcium, improved the electrophysiology, protein synthesis, andmorphology after 10 min of hypoxia (Table 1). This indicatedthat neurons could be protected against hypoxic damage even ifcalcium levels rise during hypoxia.

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Table 1. Effect of lidocaine and tetrodotoxin on damage after and cellular conditions at 10 min of hypoxia

During hypoxia the neurons slowly depolarize, reach a threshold, and then undergo a rapid depolarization to 0 mV (Hansen 1985).The reduced cellular ATP concentration during hypoxia is thoughtto inhibit the sodium-potassium pump and allow potassium to buildup outside the neuron. This would slowly depolarize the neurons,open more sodium channels, and accelerate the depolarization;lidocaine and TTX would reduce this action. Aside from the effectof depolarization on sodium channel activation, it has been demonstratedthat hypoxia can directly open sodium channels (Hammarstrom andGage 2000). This may be an important component of the slow depolarization.The hypoxic activation of these sodium channels was blocked bylidocaine and TTX (Hammarstrom and Gage 2000); these results areconsistent with our finding that lidocaine and TTX attenuate theslow depolarization, thereby delaying the onset of the rapid depolarization.It is thought that the hypoxic depolarization is an importantaspect of the pathophysiologic events (Balestrino 1995; Fung andHaddad 1997; Perez-Pinzon et al. 1998; Tanaka et al. 1997). Thereare large fluxes of sodium and calcium into the cell and potassiumout of the cell when the neurons completely depolarize (Hansen1985). There is also a massive release of glutamate, which opensligand-gated ion channels and accelerates these ion fluxes (Choi1992). The changes in cytosolic ion concentrations caused by theincreased membrane conductance are exacerbated by an inhibitionof membrane ion pumps due to decreased ATP concentrations. Itis thought that the reduced ATP and the altered cellular ionicenvironment during hypoxia triggers processes leading to delayeddamage. The current paper examines how sodium channel blockadealters the primary effects of hypoxia; it does not look at delayeddamage or secondary biochemical processes triggered by these initialchanges.

High cellular sodium levels and depolarization can have direct deleterious effects on cells. The increase in sodium can leadto cell swelling and direct histologic damage; it will also alterthe sodium electrochemical gradient and inhibit or reverse importantmembrane transporters for H⁺, Ca²⁺, and glutamate (Lipton 1999; Roettger and Lipton 1996). Sincedepolarization also affects the sodium electrochemical gradientin a similar manner, it will also affect these transporters. Thedepolarization and high cellular sodium would lead to cellularacidosis and calcium loading as well as the release of glutamateinto the extracellular space. The first two are directly damagingto cells; the release of glutamate can lead to excitotoxic damage,which is an important component of ischemic damage (Choi 1992;Lipton 1999; Siesjo and Siesjo 1996).

There is substantial evidence that increased cytosolic calcium concentrations are an important trigger for hypoxic and ischemicdamage (Kass and Lipton 1982, 1986; Roberts and Sick 1988; Siesjo1991; Tymianski and Tator 1996). Calcium is known to trigger anumber of biochemical cascades that may lead to neuronal damage(Lipton 1999; Siesjo and Siesjo 1996; Tymianski and Tator 1996).Others have also found evidence that the blockage of sodium influxcan improve recovery after hypoxia and ischemia (Astrup et al.1981; Boening et al. 1989; Lucas et al. 1989; Stys et al. 1992;Weber and Taylor 1994). It has been unclear whether this blockageof sodium influx was indirectly attenuating the rise in cytosoliccalcium by improving the pumping of calcium out of the cytosoland reducing the calcium influx by attenuating or delaying thecalcium influx through ion channels (Zhang and Lipton 1999). Inthe present study, a low concentration of lidocaine reduced thehypoxic changes in sodium and attenuated the hypoxic depolarization,but did not significantly alter the changes in ATP, calcium, orpotassium at 10 min of hypoxia. These results indicate that depolarizationand the increase in sodium during hypoxia are important triggersfor the loss of viability after hypoxia, independent of theireffect oncalcium.

We are only measuring short-term indicators of recovery; it is possible that the calcium increase during hypoxia has a greaterinfluence on delayed damage, which we cannot measure in acutebrain slices. However, a clinical study indicated that low concentrationsof lidocaine (serum levels between 16.6 and 7.8 µM) protect againstcognitive deficits, which are common after open heart surgery(Mitchell et al. 1999). These deficits are thought to be due toischemia from microemboli. We found that a low concentration oflidocaine, equivalent to 10 µM concentration used in the currentstudy, reduces infarct size 7 days after middle cerebral arteryocclusion (Lei et al. 2001). In an in vivo forebrain ischemiamodel, Liu et al. (1997) found that lidocaine improved histologicoutcome and increased the latency and reduced the amplitude ofthe extracellularly measured depolarization during ischemia. Thisis analogous to the changes we found in vitro with intracellularrecording techniques. The studies described above give us confidencethat our current study is examining mechanisms that are applicableto ischemia in vivo and long-term damage even though we can onlyexamine the acute effects of theseagents.

The length of the hypoxic depolarization correlates with damage both in vivo and in vitro (Liu et al. 1997; Perez-Pinzon etal. 1998). Both 10 and 100 µM lidocaine and 63 nM tetrodotoxindelayed the hypoxic depolarization. In addition to delaying thehypoxic depolarization, all the concentrations of lidocaine andTTX tested reduced the final level of the depolarization at 10min of hypoxia. Thus the recovery of the resting and action potentialsseem to be determined, at least in part, by the extent and magnitudeof the hypoxicdepolarization.

In support of this was the finding that 10 µM lidocaine did not improve recovery of the resting and action potentials after15 min of hypoxia; this period of hypoxia allowed the membranepotential to reach 0 mV even in the presence of 10 µM lidocaine.The membrane potential did not completely depolarize after 15min of hypoxia with 100 µM lidocaine, and both membrane and actionpotentials recovered after this period of hypoxia. In our studieswhen the membrane potential was prevented from completely depolarizing,the membrane and action potentials recover after the hypoxia.In two other studies from our laboratory, thiopental and hypothermiaattenuated the final level of depolarization during hypoxia andimproved recovery (Wang et al. 1999, 2000).

TTX (63 nM) and lidocaine (10 µM) did not significantly affect calcium but did significantly attenuate the depolarizationand reduce cellular sodium levels during hypoxia. There was improvedcell morphology, protein synthesis, and electrophysiologic recoveryunder these conditions indicating that blocking the increase insodium and the hypoxic depolarization can improve recovery evenif calcium levels still rise. This is a major finding of thispaper since most previous work emphasized the importance of calciumin leading to damage and ignored sodium'srole.

Blocking sodium channels during hypoxia has two primary effects that are difficult to separate; it reduces cytosolic sodiumlevels and attenuates the hypoxic depolarization. Both of theseeffects are significantly attenuated by concentrations of blockersthat improve recovery. We separately plotted the membrane potentialand the sodium concentration at 10 min of hypoxia versus the normalizedpercentage of protein synthesis recovery, resting potential recovery,and normal morphologic appearing neurons (type A) 1-2 h after10 min hypoxia (Fig. 10). The percentage recovery for each categorywas calculated as the value 1-2 h after hypoxia divided by itsprehypoxic value times 100. We found an inverse correlation betweenthe level of depolarization during hypoxia and the recovery ofprotein synthesis, histology, and resting potential after hypoxia(R² = 0.93, 0.68, 0.93; all slopes significantly non-zero; Fig. 10A).Protein synthesis but neither histology nor resting potentialcorrelated with sodium levels during hypoxia (R² = 0.75, 0.64, 0.44; only the slope of the protein synthesis wassignificantly different from zero; Fig. 10B). Thus an attenuationof the membrane potential during hypoxia correlates better withrecovery of the resting potential and improved morphology; interestinglyboth membrane potential and sodium concentrations correlated withimproved protein synthesis.

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Fig. 10. Effect of depolarization (mV), cellular sodium (nM/mg dry weight), and cytosolic calcium (nM) at 10 min of hypoxia on recovery after hypoxia. The membrane potential, sodium concentration, and calcium concentration at 10 min of hypoxia was plotted vs. the normalized percentage of protein synthesis recovery, resting potential recovery, and normal morphologic appearing neurons (type A) 1-2 h after 10 min hypoxia. The percentage recovery for each category was calculated as the value 1-2 h after hypoxia divided by its prehypoxic value times 100. The numbers in parentheses indicate the linear correlation coefficient (r²), the number sign indicates that the slope of the regression line was significantly different from zero. A: the less the CA1 neurons depolarize at 10 min of hypoxia the greater was the recovery of protein synthesis, histology, and resting potential after hypoxia. B: protein synthesis but not histology or resting potential correlated with sodium levels at 10 min of hypoxia. C: none of the indicators of recovery correlated with cytosolic calcium levels at 10 min of hypoxia.

Using the same analysis techniques, we demonstrated that the level of cytosolic calcium during hypoxia did not correlate wellwith protein synthesis, histology, or the resting potential (R² = 0.35, 0.13, 0.64; none of the slopes were significantly differentfrom zero). This is further evidence of protection from damagewith sodium channel blockers that is not dependent on cytosoliccalciumlevels.

A previous study (Fried et al. 1995) found that 10 µM lidocaine significantly attenuated the increase in sodium and the fallin ATP concentrations at 5 min of hypoxia, indicating that 10µM lidocaine delays the fall in ATP. Thus the changes in depolarization,sodium, and ATP may play a role in the protection by 10 µM lidocaineeven though no improvement in ATP is measured at 10 min ofhypoxia.

ATP levels fell during hypoxia; this fall was attenuated by both lidocaine and TTX. However, even untreated hypoxic tissuerecovered 60% of their prehypoxic ATP concentration by 30 minafter hypoxia (Kass and Lipton 1982; Wang et al. 1999); the energycharge recovered almost completely. ATP and energy charge arelow only during and shortly after the hypoxic period. The sodiumand potassium levels also recover substantially within 30 minof reoxygenation; sodium recovers to 118% of prehypoxic levels,and potassium recovers completely (Wang et al. 1999). Even thoughcells will not recover function as assayed by protein synthesis,histology, and recovery of the resting potential, their ATP, sodium,potassium, and calcium levels recover after hypoxia. Thus thesechanges must be triggering other events during hypoxia that leadto the damage. Our results are different from Taylor et al. (1999),who did not find recovery of the ions after in vitro ischemia.Their ischemic lesion was more severe since they not only subjectedtheir slices to hypoxia but removed glucose from the ACSF, wemaintain glucose at 4 mM during hypoxia and generate a milderlesion.

There was no further improvement in cellular morphology when the lidocaine concentration was increased from 10 to 100 µM lidocaine.This suggests that the increase in the hypoxic depolarizationand sodium were primarily responsible for the histologic damageand that calcium played only a minor role in altering cell structureshortly after hypoxia. The blockade of sodium channels would reducecell swelling and improve the histologicstate.

The alteration of protein synthesis after hypoxia may be due to the hypoxic depolarization, the increase in cytosolic sodium,and the decrease in ATP; our results indicate that calcium maynot be responsible for it. TTX (63 nM) demonstrated the same improvementof protein synthesis as 100 µM lidocaine, yet only 100 µM lidocaineblocked the increase in cytosolic calcium. TTX and lidocaine hadsimilar effects on sodium and ATPconcentrations.

Some possible mechanisms by which damage could be prevented independent of calcium are by 1) preserving ATP during hypoxia,which would improve protein synthesis and other anabolic processes;2) attenuating the hypoxic depolarization, which might block directdamage to ion channels; depolarized or inactivated channels mightbe more sensitive to damage due to proteolysis during hypoxia;and/or 3) reducing glutamate efflux by a reversed transporterand thereby attenuate excitotoxicdamage.

There was improved recovery with 100 µM compared with 10 µM lidocaine after 15 min of hypoxia; the former powerfully attenuatedthe increase in cytosolic calcium. This indicates that calciummay be an important trigger for neuronal damage. While calciumappears not to be responsible for the inhibition of protein synthesis,there is evidence that it enhances protein degradation by activatingcaspases and proteases, this will exacerbate the effects of proteinsynthesis inhibition (Lipton 1999). One hundred micromolar lidocainefurther reduced sodium and improved ATP at 10 min of hypoxia;these actions may also help explain the improved recovery with100 µMlidocaine.

Our data indicate that selective blockade of the hypoxic depolarization and the increase in intracellular sodium with a lowconcentration of lidocaine or with TTX can improve recovery afterhypoxia. This blockade improved the resting and action potentials,histologic state, and protein synthesis of CA1 pyramidal neuronsin rat hippocampal slices after 10 min of hypoxia. A higher concentrationof lidocaine, which also improved ATP, potassium, and calciumconcentrations during hypoxia, protected against more prolongedhypoxia. Thus while the depolarization and increased sodium concentrationsduring hypoxia can alone account for some of the neuronal damageafter hypoxia, changes in other components, such as calcium, ATP,and potassium also contribute to hypoxic neuronaldamage.

	ACKNOWLEDGMENTS

This work was supported by grants from the National Institute of General Medical Sciences (GM-38866) to I. S. Kass and fromthe American Heart Association, National Organization, to K. M.Raley-Susman and Heritage Affiliate to I. S.Kass.

	FOOTNOTES

Address for reprint requests: I. S. Kass, Anesthesiology Dept., Box 6, SUNY Health Science Center, 450 Clarkson Ave., Brooklyn,NY 11203-2098 (E-mail: ikass{at}netmail.hscbklyn.edu).

Received 26 April 2001; accepted in final form 17 August 2001.

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