A Novel Role of Vasopressin in the Brain: Modulation of Activity-Dependent Water Flux in the Neocortex

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The Journal of Neuroscience, May 1, 2001, 21(9):3045-3051

A Novel Role of Vasopressin in the Brain: Modulation of Activity-Dependent Water Flux in the Neocortex
Heike Niermann¹, Mahmood Amiry-Moghaddam², Knut Holthoff³, Otto W. Witte¹, and Ole Petter Ottersen²
¹ Department of Neurology, Heinrich Heine University, D-40225 Düsseldorf, Germany, ² Department of Anatomy, Institute of Basic Medical Sciences, University of Oslo, 0317, Oslo, Norway, and ³ Department of Biological Sciences, Columbia University, New York, New York 10027

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The brain contains an intrinsic vasopressin fiber system the function of which is unknown. It has been demonstrated recentlythat astrocytes express high levels of a water channel, aquaporin-4(AQP4). Because vasopressin is known to regulate aquaporin expressionand translocation in kidney collecting ducts and thereby controlwater reabsorption, we hypothesized that vasopressin might servea similar function in the brain. By recording intrinsic opticalsignals in an acute cortical slice preparation we showed thatevoked neuronal activity generates a radial water flux in theneocortex. The rapid onset and high capacity of this flux suggestthat it is mediated through the AQP4-containing astrocytic syncytiumthat spans the entire thickness of the neocortical mantle. Vasopressinand vasopressin receptor V1a agonists were found to facilitatethis flux. V1a antagonists blocked the facilitatory effect ofvasopressin and reduced the water flux even in the absence ofany exogenous agonist. V2 agonists or antagonists had no effect.These data suggest that vasopressin and V1a receptors play a crucialrole in the regulation of brain water and ion homeostasis, mostprobably by modulating aquaporin-mediated water flux through astrocyteplasmamembranes.

Key words: vasopressin; aquaporin-4; volume changes; spatial buffer; V1a receptor; intrinsic optical signals; brain water homeostasis; extracellular space

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Small vasopressin-containing neurons in the hypothalamus are known to give rise to a fiber system that extends throughoutthe brain and spinal cord (de Vries and Miller, 1998). The functionsof this intrinsic fiber system are largely unknown. One possibilityis that vasopressin controls or modulates water fluxes in thebrain, similar to its role in thekidney.

Water homeostasis in the brain is of central clinical and physiological importance. Cerebral edema is a final common pathof a number of neurological conditions and may rapidly becomelife threatening because of the rigid encasement of the brain.Furthermore, water and ion homeostasis are inextricably coupled.For example, the clearance of K⁺ from areas of high neuronal activity is contingent on a concomitantwater flux (Dietzel et al., 1980; Holthoff and Witte, 2000). Rapidtransmembrane movement of water is mediated by a distinct familyof proteins, the aquaporins, and one member of this family [aquaporin-4(AQP4)] is expressed in high amounts in brain neuropil (Nielsenet al., 1997). Knockout of AQP4 was recently found to reduce theextent of postischemic brain edema and to reduce glial swellingsecondary to hypo-osmotic stress (Manley et al., 2000).

Could vasopressin modulate aquaporin-mediated water flux in the brain? If so, this would be parallel to the situation in thekidney, where vasopressin controls water flux by regulating aquaporin-2expression and translocation. To test this hypothesis we chosea cortical slice model in which water fluxes are elicited by focalelectrical stimulation (Holthoff and Witte, 1996, 2000). Thesewater fluxes are extremely rapid, indicating that they are mediatedbyaquaporins.

Here we show that vasopressin modulates this radial, activity-dependent water flux in the cerebral cortex and that this effectis mediated through V1areceptors.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. The experiments were performed on 14-d-old male Wistar rats. Animals had free access to food and water, and institutionalguidelines for animal safety and comfort were adheredto.

Optical recording. Male Wistar rats, 14-d-old, were anesthetized and decapitated. Brains were removed rapidly and cooled downto 4°C. Coronal neocortical slices (400 µm thick) (bregma $-$ 5.8mm to bregma $-$ 6.3 mm, occipital cortex) were prepared (VT1000S,Leica) and stored at room temperature in artificial CSF (aCSF)containing (in mM): NaCl 124, NaHCO₃ 26, KCl 3, CaCl₂ 2, MgSO₄2, NaH₂PO₄ 1.25, and glucose 10, equilibrated with 95% O₂ and5% CO₂ to pH 7.4. In all experiments extracellular chloride concentrationwas reduced to 17 mM to reduce net uptake of KCl via the glialNaKCl₂ cotransporter (Dietzel et al., 1980; Holthoff and Witte,1996). This procedure ensures that most of the K⁺ uptake occurs by way of spatial buffering (Holthoff and Witte,2000). Low chloride solution contained (in mM): NaCl 10, Na-gluconate111, Ca_1/2-gluconate 4, NaHCO₃ 26, KCl 3, CaCl₂ 2, MgSO₄ 2, NaH₂PO₄1.25, and glucose 10, equilibrated with 5% CO₂ in O₂ to pH 7.4,and was washed in low chloride solution for at least 50 min beforean experiment was started. In aCSF containing tetramethylammoniumchloride(TMA-Cl), equimolar amounts of NaCl were omitted. Slices werestored in the recording chamber submerged at 32°C.

Brain slices were illuminated in the dark-field configuration of an upright microscope (Axioskop FS, Zeiss) with near-infraredlight (750 ± 50 nm) (Holthoff et al., 1994). Intrinsic opticalsignals (IOSs) (transmitted scattered light) were recorded usinga CCD camera (C2400-77, Hamamatsu). Camera signal was contrastenhanced, and shading was corrected by the CCD camera controldevice (Hamamatsu). The slices were electrically stimulated (concentricstimulation electrode, tip 100 µm; Science Products Trading) withstimulus trains (pulses of 200 µsec at 3-6 V in a train of 50Hz for 2 sec) every 10 min. Before each stimulation, backgroundintensity was captured and subtracted from actual video signal,and difference images were digitally enhanced on-line using avideo processing unit (DVS 3000, Hamamatsu). The resulting videosignal was stored on an S-VHS video recorder and analyzed off-linewith a Macintosh Computer equipped with a frame grabber card usingNIH ImageSoftware.

Double-barreled ion-selective microelectrodes. Ion-selective microelectrodes (ISMEs) were prepared with a liquid potassiumion exchanger (IE 190, WPI) and calibrated in conventional fashion.In addition to its selectivity for potassium ions, the ion exchangeris highly selective for quaternary ammonium ions (Hansen and Olsen,1980; Huang and Karwoski, 1992). Changes in extracellular space(ECS) volume can be detected by adding 10 mM TMA-Cl to extracellularfluid (Ransom et al., 1985; Huang and Karwoski, 1992). BecauseTMA is largely restricted to the extracellular compartment (Nicholsonand Phillips, 1981), changes in extracellular TMA concentrationcan be interpreted as alterations in ECS volume. In the presenceof quaternary ammonium ions, the ISMEs used are virtually blindto potassiumions.

Test agents. The following test agents were dissolved in phosphate buffer: (Arg⁸)-vasopressin (AVP; 500 nM; Bachem); [Phe², Ile³, Orn⁸]-vasopressin ([Phe², Orn⁸]-vasotocin) (500 nM; Peninsula Laboratories, Belmont, CA); (Phenylac¹, D-Tyr(Me)², Arg^6,8, Lys-NH₂⁹)-vasopressin (500 nM; Bachem); (deamino-Cys¹, D-Arg⁸)-vasopressin (500 nM, Bachem); and (D(CH₂)₅¹, D-Ile⁴, Arg⁸, Ala-NH₂⁹)-vasopressin (500 nM; Bachem). The following test agents weredissolved in dimethylsulfoxide (Merck, Darmstadt, Germany): bisindolylmaleimideI (BIS I) (300 nM, 2 µM; Calbiochem, La Jolla, CA); and thapsigargin(1 µM; ICN Biochemicals, Costa Mesa,CA).

Antibodies. Two different antibodies against AQP4 were used in this study. One was provided by Nielsen's lab in Aarhus (LL182)(Nielsen et al., 1997; Wen et al., 1999), and one was commerciallyavailable (AQP4 1A; Alpha DiagnosticsInternational).

Immunocytochemistry. The animals were anesthetized and decapitated, and neocortical slices were obtained as described above.The slices were fixed by immersion, after incubation in standardaCSF, or standard aCSF followed by aCSF with low chloride. Someslices of the latter group were exposed to 500 nM vasopressinfor 1 hr (vasopressin was added to the low-chloride aCSF). Twofixatives were used: 4% formaldehyde (for light microscopy) or4% formaldehyde/0.1% glutaraldehyde (for electronmicroscopy).

Light microscopic immunocytochemistry was performed using a method of indirect fluorescence described elsewhere (Nagelhuset al., 1999). The concentrations of antibodies were 1 or 2 µg/mlfor both antibodies. Antibodies were diluted in phosphate buffercontaining 3% normal goat serum, 1% bovine serum albumin, 0.5%Triton X-100, and 0.05% sodium azide, pH 7.4. The primary antibodieswere revealed by a carboxymethylindocyanine-coupled secondaryantibody (1:1000; Jackson ImmunoResearch Laboratories, West Grove,PA). The secondary antibody was diluted in the same solution asthe primary antibodies, with the omission of sodium azide. Thesections were viewed and photographed with a Leica Microscopeequipped with epifluorescence optics. For control the AQP4 antibodieswere omitted or preadsorbed with the immunizingpeptide.

For electron microscopic immunocytochemistry, small blocks of the cortical slices were subjected to freeze substitution (VanLookeren et al., 1991). Ultrathin sections were cut with a Reichertultramicrotome, mounted on nickel grids, and processed for immunogoldcytochemistry as described previously (Takumi et al., 1998; Wenet al., 1999). In brief, the sections were treated with a saturatedsolution of NaOH in absolute ethanol (2-3 sec), rinsed in distilledwater, and incubated sequentially in the following solutions:(1) 0.1% sodium borohydride and 50 mM glycine in Tris buffer (5mM) containing 0.01% Triton X-100 and 0.3% NaCl (TBST, 10 min);(2) 2% human serum albumin in TBST (10 min); (3) primary antibody(2.0 µg/ml both antibodies) diluted in the solutions mentionedin step 2 (overnight); (4) TBST (10 min); (5) same solution asstep 2 (10 min); and (6) gold-conjugated Fab fragments (10 or20 nm; EM.GFAR; BioCell Research Laboratories, Cardiff, UK), diluted1:20 in TBST containing 2% human serum albumin and polyethyleneglycol (0.5 mg/ml, 2 hr). Finally, the sections were examinedand micrographs were taken in a Philips CM10 transmission electronmicroscope.

Statistics. Data are given as mean ± SD. For calculation of differences, Student's t test was used. If not indicated otherwise,number of experiments equals number ofanimals.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Brain cortical slices were stimulated electrically every 10 min through an electrode in layer VI, after 50 min preincubationwith low-chloride aCSF (to prevent Cl-coupled K⁺ transport) (Holthoff and Witte, 1996). The ensuing water fluxwas assessed by recording IOSs, indicative of changes in extracellularvolume (Holthoff and Witte, 2000). Although some components ofthe IOS do not seem to correlate to the changes of extracellularspace size in extreme situations (such as spreading depression)(Aitken et al., 1999), the IOSs correlate very well with changesof extracellular space volume in the present recording and stimulusconditions (Holthoff and Witte, 1996, 2000).

The electrical stimulation caused a dark IOS (hereafter referred to as a "black wave") in the slice (Fig. 1a). Recordingsof TMA activity with ion-sensitive microelectrodes confirmed thatthe black wave corresponded to a widening of the extracellularspace (Fig. 1c) [also see Holthoff and Witte (2000)]. The wavehad a time to peak of 1.9 ± 0.4 sec (n = 9) and recovered in thecourse of the following 1-2 min. The signal started in the superficialcortical layers (I-III) perpendicular to the stimulation electrode(Fig. 1a) and expanded in the tangential plane with a velocityof 115 ± 13 µm/sec (n = 5). The area of the black wave under controlconditions varied from slice to slice (probably because of differencesin the basal level of vasopressin) with a mean ± SD of 281.53± 230.73 µm² (n = 14). The signal size was measured at its maximum after eachstimulus train. Layer IV displayed a bright signal that correspondsto a reduction of the extracellular space (as judged by TMA activityrecordings) (Holthoff and Witte, 1996, 2000). This pattern ofchanges is assumed to reflect water redistribution secondary toan activation of layer IV neurons through direct stimulation ofascending fiber systems.

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Figure 1. Effect of vasopressin on darkening of the intrinsic optical signal (black wave) corresponding to extracellular space widening. The top panels show the IOSs and field potentials evoked by afferent stimulation in the neocortical slice. Slices were electrically stimulated every 10 min with stimulus trains lasting 2 sec. Extracellular field potentials shown were recorded in layer IV and depict the response to the first stimulus within the stimulus train. IOSs were captured 6 sec after stimulation was started. The stimulation electrode in layer VI is shown schematically in this Figure. a, IOS and field potentials under control conditions. b, Increased IOS but similar field potentials after 30 min superfusion with AVP. c, Widening of extracellular space: correlation between TMA⁺ activity (left panel) and IOS (right panel). d, Statistics of field potentials under control conditions, in the presence of AVP and in the presence of a V1-antagonist. FP, Field potentials. The differences do not reach statistical significance. Scale bar, 200 µm.

AVP-treated slices

Superfusion of the slice with AVP strongly increased the areal extent of the black wave (Fig. 1b). The increase occurred inthe tangential direction; only a slight increase could be observedalong the radial axis of the cortex. AVP did not change the amplitudeof the extracellular volume increase, when assessed by TMA measurementsin the superficial cortical layers perpendicular to the stimulationelectrode. Thus the TMA concentration (Fig. 1c) (baseline, 10mM) decreased by 0.56 ± 0.4 mM in control solution (10 recordingsin slices from three animals) and by 0.68 ± 0.4 mM after AVP superfusion(9 recordings from three animals; difference not statisticallysignificant). The increase of the black wave was already apparentwith the first stimulation after solution exchange (e.g., after10 min), but reached its maximum after ~30 min. This delayed responseis probably attributable to a slow diffusion of the drug intotheslice.

The areal extent of the bright signal in layer IV (which corresponds to a reduction of the extracellular space) increasedto 368 ± 157% of control (p < 0.001; n = 9) after AVPtreatment.

Field potentials

The AVP-induced widening of the extracellular space could be secondary to changes in neuronal excitability. This was ruledout by use of extracellular field potential recordings (Fig. 1a,b,d)(n = 3). Likewise, field potentials remained unaltered after applicationof the V1a receptor antagonist (Phenylac¹, D-Tyr(Me)², Arg^6,8, Lys-NH₂⁹)-vasopressin (Fig. 1d) (n =3).

Measurement of potassium ion concentration

After electrical stimulation in layer VI, the K⁺ ion concentration increased in layer IV (where the extracellular space decreased)as well as in the superficial layers (where the extracellularspace increased) (Fig. 2a). A similar increase in K⁺ concentration was observed in slices that were stimulated inthe presence of AVP (Fig. 2b). There was no significant correlationbetween the maximal amplitude of potassium increase and the spatialextent of the black wave. The K⁺ signal had a longer duration in layer IV (24.6 ± 5.4 sec) thanin layer I (13.9 ± 4.6 sec; p < 0.02; n = 5). This duration didnot change significantly in layer I (13.5 ± 1.4 sec) or layerIV (27.1 ± 4.2 sec; recordings from five slices of three animals)after superfusion with AVP.

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Figure 2. Changes of potassium ion activity accompanying black waves. IOS and measurements of extracellular potassium ion activity in layers I and IV of the cortex under control conditions (a) and after 30 min superfusion with AVP (b). Slices were electrically stimulated every 10 min with stimulus trains lasting 2 sec. The site where the potassium activity was recorded is indicated by schematic electrodes. Scale bar, 200 µm.

V1 and V2 receptors

[Arg⁸]-vasopressin (Fig. 3a) (n = 9) and the V1 agonist [Phe², Orn⁸]-vasotocin (n = 3) increased the size of the black wave by >50%(Fig. 3b). Signal sizes were determined after 40 min of drug application.The V1 antagonist decreased the size of the black wave (Fig. 3b)(n = 3), i.e., without addition of AVP. This indicates that endogenousV1 agonists exert a tonic facilitatory effect. The V2 agonist[deamino-Cys¹, D-Arg⁸]-vasopressin, and the V2-antagonist [d(CH2)₅¹, D-Ile², Ile⁴, Arg⁸, Ala-NH₂⁹]-vasopressin did not affect the size of the black wave (Fig.3b) (n = 3).

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Figure 3. Pharmacological influences on the size of the black wave. Slices were electrically stimulated every 10 min with stimulus trains lasting 2 sec. a, Typical experiment with application of AVP. After three control stimulations the slice was superfused with AVP, which caused an increase of the black wave. b, Statistics of effects of AVP, the V1-agonist [(Phe², Ile³, Orn⁸)]-vasopressin [(Phe², Orn⁸)-vasotocin], the V2 agonist (deamino-Cys¹, D-Arg⁸)-vasopressin, the V1-antagonist Phenylac¹, D-Tyr(Me)², Arg^6,8, Lys-NH₂⁹)-vasopressin, and the V2-antagonist [D(CH₂)₅¹, D-Ile⁴, Arg⁸, Ala-NH₂⁹]-vasopressin on the maximal extension of the black wave. Signal sizes were determined after 40 min of drug application. V2 agonists or V2 antagonists did not affect the size of the black wave. The difference between values for AVP and V1 agonist is not statistically significant (p > 0.05), but both values (and the value for the V1 antagonist) differ from control level (dashed line) and all other observations (p < 0.05). In this and the following Figures the signal size was expressed in arbitrary areal units as measured on-screen.

Thapsigargin and protein kinase C

To test for the role of intracellular calcium stores, thapsigargin (1 µM), which inhibits the endoplasmic reticulum Ca²⁺ ATPase and prevents a refill of the Ca²⁺ stores (Norup et al., 1986), was washed for 60 min. This decreasedthe size of the black wave evoked by afferent stimulation (Fig.4a,b) (n = 3). In the presence of thapsigargin, AVP no longerhad a facilitatory effect (Fig. 4b) (n = 4). Sometimes a rundownof signal size was observed with recording times exceeding 90min. Figure 4c shows that no such rundown was present within thefirst 90 min that were used for the experiments in the presentstudy.

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Figure 4. Changes of IOS sizes after superfusion with thapsigargin. Slices were electrically stimulated every 10 min with stimulus trains lasting 2 sec. a, Thapsigargin decreased the amplitude of the black wave. Three control stimulations were followed by superfusion with thapsigargin for 60 min. b, In the presence of thapsigargin, AVP did not restore or enhance the black wave. Comparison between thapsigargin (60 min after onset of superfusion) and thapsigargin for 30 min followed by thapsigargin plus AVP for 30 min. There was no significant difference (p > 0.05); however, both values differed from control level (dashed line) at p < 0.05. c, Absence of rundown in a typical control experiment with electrical stimulation every 10 min for 90 min. d, Effects of different concentrations of bisindolylmaleimide I (BIS I) together with AVP (500 nM) on size of the black wave. Signal sizes were determined after 60 min of application. There was no significant difference between the two concentrations (p > 0.05); however, both values differed from control level (dashed line) at p < 0.05.

To test whether the effect of AVP is mediated through protein kinase C (PKC), the PKC-inhibitor BIS I was given simultaneouslywith AVP (500 nM) in two different concentrations. BIS I blockedthe enhancing effect of AVP and decreased the black wave to belowcontrol levels when added at a concentration of 2 µM (n = 5) or300 nM (n = 4) (Fig. 4d). Signal sizes were determined after 60min of drugapplication.

Immunocytochemistry

Immunofluorescence of cortical slices treated with AVP revealed intense AQP4 immunolabeling associated with the pial surfaceand blood vessels (Fig. 5a,b). This pattern of immunolabelingwas indistinguishable from that of control slices (data not shown).Extracerebral vessels were consistently unlabeled (Fig. 5b). Thisis in agreement with the immunogold data (Fig. 5c), which showthat AQP4 is expressed by perivascular glial processes but notby endothelial cells. High particle densities were also observedalong the glial plasma membranes apposed to pia (data not shown).Other domains of astrocyte plasma membranes were labeled at lowerintensities. The pattern of immunolabeling in immersion-fixedcortical slices did not differ from that in perfusion-fixed brain(Fig. 5d). No immunofluorescence or immunogold signals were observedin the absorption controls (data not shown).

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Figure 5. a, b, Immunofluorescence labeling of AQP4 in a cortical slice treated with vasopressin. a, Strong AQP4 immunolabeling of the glia limitans (double arrows) facing the unlabeled pia, and of glial end feet surrounding the blood vessels (short arrows). p, Pia. b, Higher magnification showing an unlabeled pial vessel (arrow). Scale bar, 20 µm. c, d, Immunogold labeling of AQP4. c, AQP4 labeling of glial end feet surrounding a collapsed vessel in a cortical slice treated with vasopressin. d, Electron micrograph showing AQP4 labeling of glia limitans facing a pial vessel in rat parietal cortex. V, Vessel lumen; B, basal lamina; G, glial process. Scale bar, 0.3 µm.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

High neuronal activity generates excess K⁺ that has to be efficiently cleared from the synaptic region. Dissipation throughthe narrow extracellular space is clearly insufficient (Dietzelet al., 1980), calling for a role of the astroglial syncytiumthat occupies most of the space between cerebrocortical neurons.Astrocytes are equipped with several mechanisms for K⁺ handling, the most important of which is K⁺ spatial buffering. This mechanism can be studied in relativeisolation depending on the experimental conditions. Notably, inthe present series of studies the low [Cl] in the incubation medium should prevent any activation of theNaKCl₂ transporter (Holthoff and Witte, 1998).

It has long been known that K⁺ spatial buffering generates osmotic gradients and that these have to be compensated by waterredistribution (Dietzel et al., 1980). One piece of evidence forthis is the shrinkage of the extracellular space that occurs aroundactive neurons. It follows that any K⁺ flux through glial syncytia must be associated with a directionallyspecific water flux (Holthoff and Witte, 2000). This was borneout in the present study. Thus, evoked activity in the deep corticallayers elicited a flux of K⁺ to the superficial layers of the cortex (as measured by K⁺-sensitive microelectrodes), and this flux was accompanied bya water flux (recorded as an enlargement of the extracellularspace). This water flux originated around the active neurons inlayer IV, as indicated by the shrinkage of the extracellular spaceat this site. The volume changes in the deep and superficial corticallayers occur with a delay of <2 sec after electrical stimulation.The faster dissipation of potassium in upper cortical layers mayreflect loss through the cortical surface. Rapid transmembranewater transport seems to be mediated by a specialized class ofchannel molecules, the aquaporins (Agre et al., 1995). AQP4 occursin high concentrations in brain (Jung et al., 1994). Recent studiesshowed that this aquaporin is largely restricted to astrocytes,implying that it should be uniquely suited to facilitate watertransport coupled to K⁺ spatial buffering (Nielsen et al., 1997; Nagelhus et al., 1998).Here we demonstrate that AQP4 is expressed by cortical astrocytesand that their expression pattern is maintained in the corticalslicepreparation.

The present experimental approach is based on the idea that evoked K⁺ fluxes can be used to drive AQP4-mediated water transport. Evenif high frequency stimulation is used, our approach is likelyto mimic the physiological situation much more closely than alternativeprocedures based on cultures or cell lines challenged with hypo-osmoticor hyperosmotic media. What is lost in the present model comparedwith the in vivo situation is the access to the blood stream andsubarachnoidal space, which are believed to be the ultimate sinksof excess K⁺. However, when using IOSs as a measure of water transport, leavingout the ultimate sinks is turned to an advantage because thisis likely to accentuate the volume changes of the extracellularspace.

Here we tested our hypothesis that vasopressin may exert an important regulatory role on brain water transport. Vasopressinwas chosen for the following reasons. First, vasopressin is endogenousto the brain (Landgraf, 1992), and the brain has an intrinsicvasopressin-containing fiber system (Buijs, 1978; de Vries andMiller, 1998). Second, V1 vasopressin receptors are widely distributedthroughout the cerebral cortex (Chen et al., 1993; Brinton, 1999).Third, vasopressin increases the rate of osmotically induced volumechanges of astrocytes in culture (Sarfaraz and Fraser, 1999).Our results are compatible with the following scheme. K⁺ released consequent to the evoked neuronal activity accumulatesin the extracellular space of layer IV. Some of this K⁺ is cleared by spatial buffering. In the presence of AVP, watertransport through astrocytes will be facilitated, allowing thecells to better compensate for the osmotic gradients set up byK⁺ transport. In other words, vasopressin will enable a radial waterflux even lateral to the stimulating electrode, where the evokedneuronal activity is lower and the potassium driving force smallerthan in the cortex perpendicular to the site of stimulation. Thiswill be recorded as an enhanced tangential spread of the IOS inthe superficial as well as in the deep layers of the cortex (representingan increase and decrease, respectively, of the extracellular spacevolume). In agreement with the involvement of the glial syncytium,pharmacological decoupling of the glial cells abolishes the wideningof the extracellular space in superficial cortical layers (Holthoffand Witte, 2000).

V1a receptors and water redistribution

The present data indicate that the effect of vasopressin is mediated through V1a receptors rather than V2 receptors. Preincubationwith a V1a antagonist caused a decrease in the black wave evenunder basal stimulation conditions (i.e., in the absence of anyother drugs in the medium). These data suggest that there is atonic, V1a receptor-mediated facilitation of water permeability.This tonic stimulation could be provided by AVP released fromnerve fibers intrinsic to the cerebral cortex (Sofroniew, 1983)or by AVP diffusing into the cortex via the extracellular space.In vivo the extracellular AVP level may reach nanomolar levels(Robinson, 1983; Landgraf, 1992), attesting to the physiologicalrelevance of the present AVP concentration. Local vasopressinrelease in brain tissue is increased by high K⁺ (Landgraf, 1992).

Intracellular signaling mechanisms

The V1a receptors are coupled via G-proteins to phospholipase C (Thibonnier et al., 1994). Thus one possibility is that theeffects of V1a stimulation on extracellular volume are mediatedthrough an IP3-dependent release of Ca²⁺ from internal stores. In support of this we could demonstratethat a depletion of these stores by use of thapsigargin abolishedthe facilitatory effect of vasopressin on waterredistribution.

V1a receptor stimulation also causes activation of PKC. By use of a PKC inhibitor (BIS I together with AVP), evidence wasprovided that vasopressin exerts part of its facilitatory effectthrough this signaling pathway. With a BIS I concentration of300 nM and 2 µM (which would inhibit all major PKC subtypes),a reduction of the black wave was observed. The signals becameeven smaller than under control conditions, possibly relatingto the fact that the effects of the basal level of vasopressinwere also antagonized by the inhibitor. This is in contrast tothe observation of Yang and Verkman (1997), who found no changein AQP4 activity after PKC activation. However, the latter studywas performed in oocytes that may have different PKC isoformsor PKC substrates. It remains to be shown whether PKC acts throughphosphorylation of AQP4 or, more indirectly, through phosphorylationof one or several molecules upstream in the signal transductionpathway. AQP4 is known to contain three putative phosphorylationsites, and studies are under way to resolve whether these aretargeted by V1 receptorstimulation.

That vasopressin has some effects on other membrane proteins cannot be excluded. In fact, in the absence of specific blockersthere is as yet no direct evidence that the observed effects aremediated by aquaporin-4. An involvement of gap junctions is unlikely.PKC reduces gap junction conductance (Greenfield et al., 1990),and intracellular calcium, at least at high concentrations, decreasesjunctional permeability (Blomstrand et al., 1999). This contrastswith our findings that both PKC and intracellular calcium areinvolved in the facilitation of waterredistribution.

Does vasopressin alter the expression pattern of AQP4?

So far we have tacitly assumed that any regulation of AQP4-mediated water flux must be caused by an allosteric modulationof the AQP4 channel. However, there is an alternative possibility:namely, that the changes in water permeability are caused by alterationsin AQP4 expression. The latter idea is not supported by the presentimmunocytochemical analysis, which failed to provide any evidenceof a vasopressin-induced translocation of AQP4 to the plasma membrane.In fact, similar to the situation in other cell populations (Nielsenet al., 1997), most of the AQP4 molecules in cortical astrocytesare located at the cell surface even in basal conditions. In contrast,our immunogold data cannot rule out the possibility that vasopressincauses a subtle reorganization of the plasma membrane AQP4 moleculeswithin the individual membrane compartments. A combined freeze-fracture/immunogoldapproach (Rash et al., 1998) would be required to settle thisissue.

Conclusion

Our data are consistent with the idea that vasopressin through V1a receptors facilitates an activity-dependent flux of waterthrough the cortical astrocyte syncytium. The rapid time courseof the volume changes suggests that the effect of vasopressinis mediated by modulation of a specialized water channel, mostprobably aquaporin-4. In vivo, the efflux pathway described herewill be interfaced to extracerebral fluid spaces. Because waterflux through AQP4 is osmotically driven, this pathway will alsoadmit water movement in the opposite direction. In fact, it isknown that vasopressin causes a net increase in brain water content,accompanying a net electrolyte accumulation (DePasquale et al.,1989). An important task for further studies will be to resolvewhether the present regulatory mechanisms may be useful therapeutictargets in brainedema.

  FOOTNOTES

Received Oct. 26, 2000; revised Jan. 16, 2001; accepted Jan. 23, 2001.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB 194 and 1849), the Düsseldorf Entrepreneurs Foundation,the Norwegian Research Council, and the Letten F. Saugstad's Foundation.We thank C. Bruehl and K. Schiene for helpful discussions andS. Hamm, D. Steinhoff, and Milan Srejic for technicalassistance.
H.N. and M.A.-M. contributed equally to thispaper.

Correspondence should be addressed to Prof. Dr. Otto W. Witte, Neurologische Klinik, Heinrich Heine Universität, Moorenstrasse5, D40225 Düsseldorf, Germany. E-mail: witteo{at}uni-duesseldorf.de.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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