Global Loss of Na,K-ATPase and Its Nitric Oxide-Mediated Regulation in a Transgenic Mouse Model of Amyotrophic Lateral Sclerosis

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The Journal of Neuroscience, January 1, 2003, 23(1):43-51

Global Loss of Na,K-ATPase and Its Nitric Oxide-Mediated Regulation in a Transgenic Mouse Model of Amyotrophic Lateral Sclerosis
Dorette Z. Ellis, Jason Rabe, and Kathleen J. Sweadner
The Neuroscience Center, Massachusetts General Hospital, Charlestown, Massachusetts 02129

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Na,K-ATPase plays a critical role in energy metabolism and ion fluxes. Its loss was investigated in the G93A mouse model ofamyotrophic lateral sclerosis (ALS) in which the mutation of Cu/Znsuperoxide dismutase (SOD1) is thought to lead to aberrant oxidativedamage. Observed losses in spinal cord Na,K-ATPase activity exceededall expectations. All three catalytic subunit isoforms ( $alpha$ 1, $alpha$ 2, $alpha$ 3) were reduced, and the global $alpha$ subunit loss affected not justneurons, glia, and myelinated axon tracts but even ependymal andpial membranes. Decreases in Na,K-ATPase activity were greaterthan losses of protein, and there were losses of Na,K-ATPase $alpha$ ,but not $beta$ , subunits. Together, these observations are consistentwith selective degradation of the $alpha$ subunit after damage. Overexpressionof normal SOD1 does not cause ALS-like symptoms, but it has otherknown pathological effects. In transgenic mice overexpressed normalhuman SOD1 had a smaller but still considerable effect on Na,K-ATPase.Furthermore, the nitric oxide-mediated regulatory pathway forNa,K-ATPase inhibition was undetectable in spinal cord tissueslices from mice overexpressing either mutant or normal humanSOD1. Na,K-ATPase activity did not respond to nitric oxide donors,and the free radical-dependent step of the pathway could not bebypassed by the addition of the downstream protein kinase G activator,8-Br-cGMP. The data demonstrate that Na,K-ATPase is vulnerableto aberrant SOD1 activity, making it a potential contributingfactor in disease pathology. Moreover, the global cellular distributionof Na,K-ATPase loss indicates that SOD1 overexpression is far-reachingin its pathologicaleffects.

Key words: Na,K-ATPase; SOD1; amyotrophic lateral sclerosis; neurodegeneration; spinal cord; nitric oxide

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Amyotrophic lateral sclerosis (ALS) is an age-dependent motor neuron disease. Certain familial ALS cases are inherited asan autosomal dominant trait with mutations in cytosolic Cu/Znsuperoxide dismutase 1 (SOD1) (Rosen et al., 1993; Brown, 1995).SOD1 normally converts superoxide, a by-product of mitochondrialmetabolism, to water and hydrogen peroxide. Simple loss of SOD1activity has been ruled out as a cause of the disease. Instead,there is evidence for "gain of toxic function," such as increasesin copper-, free radical-, or oxidative damage, which is not alleviatedby increases or decreases in the level of normal SOD1 activity(Cleveland and Rothstein, 2001; Julien, 2001).

The Na,K-ATPase consumes 50% of the energy supply in the CNS (Ames, 2000). Its catalytic ( $alpha$ ) subunit is sensitive to damageby free radicals and other oxidative stress (Kim and Akera, 1987;Xie et al., 1995; Mense et al., 1997), and the oxidized Na,K-ATPase $alpha$ subunit can be degraded by calpain, proteosomal, and lysosomalpathways (Zolotarjova et al., 1994; Thevenod and Friedmann, 1999).It thus may be one of the links between alterations in free radicalhomeostasis and ALS pathology. In other circumstances the inhibitionof Na,K-ATPase increases the sensitivity of neurons to glutamateexcitotoxicity because of complementary effects on neurons (enhancingglutamate effects and Ca²⁺ accumulation) and astrocytes (reducing the driving force forNa⁺-dependent glutamate clearance) (Lees et al., 1990; Brines andRobbins, 1992; Brines et al., 1995; Calabresi et al., 1995; Leesand Leong, 1996; Stelmashook et al., 1999). Furthermore, the freeradical nitric oxide (NO·) normally regulates the Na,K-ATPasevia the activation of soluble guanylate cyclase and cGMP (McKeeet al., 1994), a pathway that is shared by glutamate and oxygenfree radicals in the CNS. This pathway forms a convergence pointfor the action of several intercellular and intracellular molecularmessengers that have been implicated in neuronal viability understress (Dawson et al., 1991; Nathanson et al., 1995). Together,these suggest that either loss or excessive inhibition of Na,K-ATPasecould contribute to motor neuron death via direct oxidative damageor via the enhancement of NO· and other free radicaleffects.

The Na,K-ATPase has two required subunits, $alpha$ and $beta$ . There are three $alpha$ isoforms ( $alpha$ 1, $alpha$ 2, and $alpha$ 3) and three $beta$ isoforms ( $beta$ 1, $beta$ 2, and $beta$ 3) in the CNS (Sweadner, 1989; Blanco and Mercer, 1998),which have different kinetic properties and are likely to be regulateddifferently (Blanco and Mercer, 1998; Crambert et al., 2000).Although there are many exceptions to the rule, neurons have predominantly $alpha$ 3 $beta$ 1 and astrocytes have predominantly $alpha$ 2 $beta$ 2, whereas both neuronsand glia can express $alpha$ 1.

To test the hypothesis that Na,K-ATPase loss occurs in a mouse model of ALS and in SOD1 overexpression, we used transgenicmice that express either human SOD1 with the G93A missense mutationor normal human SOD1 over and above normal mouse SOD1 (Gurneyet al., 1994).

  Materials and Methods

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Reagents. Routine reagents, sodium nitroprusside (SNP), superoxide dismutase, and ouabain were purchased from Sigma (St. Louis,MO). ¹H-[1,2,4]oxadiazolo[4,3-a]quinoxalin-1-one (ODQ), diethylenetriamineNO (DETA-NO), 8-Br-cGMP, and okadaic acid were obtained from Sigma-RBI(Natick, MA). The cGMP enzyme immunoassay system was purchasedfrom Amersham Biosciences (Piscataway, NJ). Cy3-conjugated goat-antimouse IgG was purchased from Jackson ImmunoResearch Laboratories(West Grove, PA). The Puregene DNA Isolation Kit was purchasedfrom Gentra (Minneapolis,MN).

Transgenic SOD1 mice. The mice were obtained from Dr. Robert H. Brown Jr. (Massachusetts General Hospital, Charlestown, MA)or The Jackson Laboratory (Bar Harbor, ME) and were strains originallydeveloped by Dr. Mark Gurney (Gurney et al., 1994). The G1H strainof G93A mice carries high copy numbers of human SOD1, with a missensemutation substituting glycine with alanine at codon 93, and developsALS-like symptoms between 3 and 4 months of age. This strain ismaintained as a hemizygote hybrid line, progeny of a cross betweenC57BL/6J and SJL mice. Transgenic males were crossed with nontransgenicB6SJL-F1 females. Animals were genotyped by purifying mouse tailDNA with a Puregene DNA Isolation Kit; PCR products were separatedon a 2% agarose gel. The controls were transgenic normal humanSOD1 overexpressors of the B5SJL strain and nontransgeniclittermates.

Na,K-ATPase activity and cGMP measurements. Whole spinal cord tissue was dissected, and tissue slices (0.4 × 0.4 × 1 mm) wereprepared on a Brinkmann chopper cooled to 4°C and suspended (25-30mg/ml wet weight) in microdissection buffer containing (in mM):137 NaCl, 5 KCl, 0.8 MgSO₄, 0.25 CaCl₂, 1.0 MgCl₂, 10 HEPES, and2 NaOH, pH-adjusted to 7.4 at 34°C.

SNP, DETA-NO, or 8-Br-cGMP, when used, was added to tubes that contained 1 ml aliquots of slice suspension. Tubes were incubatedfor 15 min at 34°C with rocking and then frozen at -80°C. In studiesthat used ODQ or okadaic acid, the inhibitor was added 3 min beforethe addition of the other drug. Tubes were thawed and centrifuged(1700 × g for 15 min at 4°C), and the supernatant was removedand assayed for cGMP by using an enzyme immunoassay accordingto the manufacturer's instructions. The tissue slice pellets wereresuspended in resuspension buffer containing (in mM): 85 NaCl,20 KCl, 4 MgCl₂, 0.2 EGTA, and 30 histidine, pH-adjusted to 7.2.

Two similar ATPase assays were used. For most experiments with tissue from 4-month-old animals the Na,K-ATPase activity wasdetermined by using the pyruvate kinase/lactate dehydrogenaseassay that couples the generation of ADP and oxidation of NADHas described previously (Ellis et al., 2000). Treated tissue sliceswere homogenized with a ground glass homogenizer. Na,K-ATPaseactivity was calculated from the difference between the slopesin the time course of absorption change at 340 nm in the absenceand the presence of 3 mM ouabain. For most experiments with tissuefrom 2-month-old animals the activity was determined by the colorimetricATPase assay: ATP was hydrolyzed, and the released P_i was measuredby forming a complex with molybdate. The pelleted tissue sliceswere resuspended and refrozen for at least 20 min at -80°C in1 ml of resuspension buffer. Tubes were thawed on ice water. Forfurther permeabilization saponin (20 µg/ml) was added, and theslices were incubated for 10 min at 34°C. Aliquots of tissue slices(~10-15 µg; 7.5-10 µl) were added to 300 µl of ATPase buffer containing(in mM): 3 ATP, 140 NaCl, 20 KCl, 3 MgCl₂, and 30 histidine, pH7.2, with or without 3 mM ouabain. In this and previous work weverified the equivalence of the two assays that were used (Elliset al., 2000).

Immunoblots. Spinal cord tissue was dissected from transgenic mutant SOD1 mice, transgenic normal human SOD1 overexpressors,and nontransgenic littermate controls and then homogenized at4°C in microdissection buffer. Protein concentrations were determinedby the Lowry method, and samples (50 µg of protein) were separatedby gel electrophoresis on Laemmli gels and transferred to nitrocellulosemembrane electrophoretically. For detection of Na,K-ATPase subunitsthe isoform-specific monoclonal antibodies used were 6F (for $alpha$ 1;Developmental Studies Hybridoma Bank, Iowa City, IA), McB2 (for $alpha$ 2), and XVI-F9G10 (for $alpha$ 3; Affinity BioReagents, Neshanic Station,NJ), all of which bind in the first 60 residues of the respective $alpha$ subunits; rabbit polyclonal antibodies SpETb1 and SpETb2 (giftof P. Martin-Vasallo, University of Tenerife, Spain) were usedfor $beta$ 1 and $beta$ 2, respectively. Anti-KETYY against the $alpha$ C terminus(gift of Dr. J. Kyte, University of California, San Diego, CA)was used to detect all $alpha$ isoforms together. Anti-superoxide dismutase(Cu/Zn) polyclonal antibody specific to human SOD1 (Calbiochem-Novabiochem,San Diego, CA) was used to quantify the level of overexpressedenzyme. Blots subsequently were stained with horseradish peroxidase-conjugatedsecondary antibody, developed with luminol reagent, and quantifiedwith a Molecular Dynamics scanning densitometer (Sunnyvale,CA).

Immunofluorescence. Nontransgenic controls and transgenic mutant SOD1 mice were anesthetized and perfused with PBS, followedby periodate-lysine-paraformaldehyde fixative for 20 min (McLeanand Nakane, 1974). The spinal cords encased in the vertebral columnswere harvested and postfixed for 48 hr. The spinal cords wereremoved and washed in PBS overnight and then soaked in 25% sucrosein 0.1 M PBS for 24 hr before sectioning. Cryostat sections (10-14µm) were cut at $-$ 20°C and collected on positively charged slides(ProbeOn Plus, Fisher Scientific, Durham, NC). Slides were washedin 0.1 M PBS and incubated in blocking buffer containing 0.1%Triton X-100 and 5% normal goat serum in PBS. Tissue sectionswere incubated with primary monoclonal antibodies for the $alpha$ subunitsdescribed above, washed, and stained with secondary antibody Cy3-conjugatedgoat-anti mouse IgG. For $beta$ 1, monoclonal antibody BSP-3 was used,a gift of Dr. C. Goridis (INSERM-CNRS, Marseille Luminy, France).For $beta$ 2, monoclonal antibody 426 was used, a gift of Dr. MelittaSchachner (University of Hamburg, Germany). The images were viewedwith a Zeiss confocal microscope (Oberkochen,Germany).

Statistics. Statistical comparisons were performed by ANOVA, followed by Fisher's protected least significant difference (PLSD)and Scheffé's F test for comparison of significant differenceamong differentmeans.

  Results

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ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Decreased ouabain-sensitive Na,K-ATPase activity in transgenic mutant SOD1 mice

Ouabain-sensitive Na,K-ATPase activity was measured in spinal cord tissue slice homogenates of transgenic mice expressingmutant or normal human SOD1 and wild-type controls. Because theassay is performed in vitro with saturating levels of ATP andions, the measured activity reflects the maximal velocity of theenzyme itself and not ATP depletion secondary to mitochondrialdamage in vivo. Figure 1A shows that Na,K-ATPase activity wasdecreased remarkably (70-75%) in the severely impaired 4-month-oldmutant SOD1 mice compared with nontransgenic animals. To determinewhether the decreases were a result of the mutation or of overexpressionof SOD1, we measured activity in samples from transgenic miceoverexpressing normal human SOD1. There was a large but less dramaticdecrease (40-45%) in ouabain-sensitive Na,K-ATPase activity inthe overexpressors. Immunoblot and densitometric analysis witha species-specific antibody for human SOD1 showed that the totallevel of exogenous SOD1, compared with a sample of purified enzyme,was not statistically different in mice overexpressing mutantand normal human SOD1 (Fig. 1B,C). The greater Na,K-ATPase activityloss in the mutant is consistent with "gain of function" consequencesof excess SOD1 that are exacerbated by the mutation.

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Figure 1. Ouabain-sensitive Na,K-ATPase activity in spinal cord and cerebellum of nontransgenic controls (Control), transgenic normal human SOD1 overexpressors (SOD++), and transgenic SOD1 mice (Mutant), and expression of normal and mutant human SOD1. For A and D, activity is expressed as µmol P_i/hr per milligram of protein. A, Spinal cord tissue slices from 4-month-old animals were homogenized, and ouabain-sensitive Na,K-dependent hydrolysis of ATP was determined. Values for activity represent the means ± SEM for an average of three samples in five experiments. *Significantly different from control at p < 0.05 (by ANOVA, Fisher's PLSD, and Scheffé's F test). ^#Significantly different from transgenic normal human SOD1 overexpressors at p < 0.05 (by ANOVA and Fisher's PLSD). B, Immunoblot detection of human SOD1 in nontransgenic controls (lane 2), transgenic mutant SOD1 mice (lane 3), normal human SOD1 overexpressors (lane 4), and purified human SOD1 as a positive gel control (lane 1). C, Densitometric analysis of human SOD1 expression levels in transgenic mutant SOD1 mice (Mutant), transgenic normal human SOD1 overexpressors (SOD++), and purified human SOD1 as a positive gel control. Values are expressed as arbitrary units and represent the means ± SEM for an average of three experiments. D, Na,K-ATPase activity was measured from cerebellar tissue slices from 4-month-old animals. Values represent the means ± SEM for an average of three samples in six experiments. *Significantly different from control at p < 0.05 (by ANOVA, Fisher's PLSD, and Scheffé's F test). E, Na,K-ATPase activity was measured in spinal cord tissue slice preparations from 2-month-old animals. Values for ouabain-sensitive Na,K-ATPase activity represent the means ± SEM for an average of three samples in three experiments.

Cerebellum is not implicated in neurodegenerative processes in this ALS mouse model (Almer et al., 1999), but comparable lossesin Na,K-ATPase activity also were seen in cerebellum in 4-month-oldanimals (Fig. 1D). In agreement with Almer et al. (1999), we didnot see any indication of major neuron loss in cerebellar tissuesections (data not shown). This is an initial indication thatthe losses of activity were not attributable simply to a lossof neurons. Figure 1E shows that there were no significant reductionsin Na,K-ATPase activity in spinal cord of transgenic mutant miceor transgenic overexpressors at 2 months of age, before the onsetof obvious neurologicalsymptoms.

Decreased Na,K-ATPase $alpha$ subunits in transgenic mutant SOD1 mice

Losses in Na,K-ATPase activity could be attributable to enzyme inactivation, protein degradation, changes in gene expression,failure to transport newly synthesized protein to the axon, lossof neurons, or a combination of these. Quantitative detectionof Na,K-ATPase subunits makes it possible to assess whether proteinlevels were changed as much as activity. It also allows some conclusionsto be made about whether the effect is on a particular Na,K-ATPaseisoform or a particular cell type, because the $alpha$ 3 subunit is allin neurons and the myelinated axon tracts, whereas most of $alpha$ 2is in astrocytes (Hieber et al., 1991; McGrail et al., 1991; Wattset al., 1991; Peng et al., 1997). The relative content of Na,K-ATPase $alpha$ 1, $alpha$ 2, and $alpha$ 3 subunits was determined in homogenates of spinalcord of transgenic mutant SOD1 mice, transgenic normal human SOD1overexpressors, and nontransgenic controls by using isoform-specificmonoclonal antibodies. Immunoblots (Fig. 2A) and densitometricanalysis (Fig. 2B) showed that there were decreases in $alpha$ 1 (65%), $alpha$ 2 (50%), and $alpha$ 3 (50%) in transgenic mutant SOD1 mice comparedwith nontransgenic controls. Although there were also decreasesin the three $alpha$ isoforms in transgenic normal human SOD1 overexpressors,the decreases were smaller compared with transgenic mutant mice(Fig. 2B). Total Na,K-ATPase $alpha$ subunit level was quantified witha polyclonal antibody, anti-KETYY, that recognizes all Na,K-ATPaseisoforms. Figure 2, C and D, shows that there were close to 50%decreases in total $alpha$ protein in transgenic mutant SOD1 mice whencompared with nontransgenic controls and 20-25% decreases in normalSOD1 overexpressors. Isoform-specific antibodies for the $beta$ 1 and $beta$ 2 Na,K-ATPase subunits were used to examine $beta$ levels. In contrastto the $alpha$ subunit, no differences were detected in $beta$ 1 (mostly inneurons) or $beta$ 2 (mostly in astrocytes) in spinal cord samples fromtransgenic mutant SOD1, transgenic normal human SOD1 overexpressors,or nontransgenic control animals (Fig. 2E). $beta$ 3, which is foundonly in oligodendrocytes and at a low level (Martin-Vasallo etal., 2000), was not examined.

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Figure 2. Immunoblot detection and quantitative analysis of Na,K-ATPase isoforms in nontransgenic controls (C, control), transgenic mutant SOD1 mice (M, mutant) and transgenic normal human SOD1 overexpressors (O, SOD++). A, B, Immunoblot and densitometric analysis of $alpha$ 1, $alpha$ 2, $alpha$ 3. For all immunoblots 50 µg of spinal cord homogenates was used. A, Separated protein was stained with monoclonal antibodies to $alpha$ 1 (6F), $alpha$ 2 (McB2), and $alpha$ 3 (XVIF9G10). Crude homogenates from rat brain served as positive controls for the antibodies (data not shown). Molecular weight markers are shown in kDa. B, Data are expressed as arbitrary units and represent the means ± SEM for an average of three experiments. C, Immunoblot stained with KETYY, an antibody that recognizes all Na,K-ATPase $alpha$ subunits. D, Densitometric analysis of KETYY expressed in arbitrary units and representing the means ± SEM for an average of three experiments. E, Spinal cord homogenates were stained for $beta$ 1 (SpETb1) and $beta$ 2 (SpETb2) polyclonal antibodies. The data that are shown are representative of multiple experiments.

The reduction in Na,K-ATPase activity (Fig. 1A) exceeded the reduction in total Na,K-ATPase $alpha$ subunit (Fig. 2D) in both mutantSOD1 mice and normal human SOD1 overexpressors by a substantialamount. Both measures were expressed per milligram of protein,and so the losses were over and above any generalized loss oftissue mass, which does occur with the loss of motor neurons.The greater loss of ATP hydrolysis than $alpha$ subunit indicates thatperturbations of SOD1 activity have an acute effect on Na,K-ATPaseapart from any effect on gene expression, tissue or axon atrophy,or cellloss.

Na,K-ATPase isoform distribution in normal and mutant spinal cord

The distribution of the various Na,K-ATPase $alpha$ subunits was determined by using confocal immunofluorescence with isoform-specificmonoclonal antibodies. In the dorsal horn of the rat spinal cordsome large neurons express both $alpha$ 2 and $alpha$ 3, whereas in the ventralhorn some motor neurons express $alpha$ 1 and $alpha$ 3 and the rest just $alpha$ 3(Mata et al., 1991; McGrail et al., 1991; Watts et al., 1991).In the mice that were investigated here, the pattern of stainingfor each $alpha$ isoform was identical in sections from all levels ofthe spinal cord (cervical, thoracic, lumbar, and sacral; datanot shown) except for the underlying structural differences indorsal and ventral horns and axon tracts at different levels.Figure 3 shows immunostaining of tissue sections from the lumbarexpansion of the spinal cord in 4-month-old nontransgenic controlsand transgenic mutant SOD1 mice. In keeping with the plasma membranelocation of the Na,K-ATPase, the cytoplasm of large-diameter neuronalcell bodies was unstained, although there were $alpha$ 3 ring-stainedcell bodies in the central and lower regions of the dorsal horn. $alpha$ 2 stain characteristic of astrocytes was brightest in the graymatter, but it extended outward into the myelinated tracts accompanyingradiating bundles of axons. It was notable that there were differencesin the distribution of Na,K-ATPase isoforms in wild-type mousespinal cord that have not been described before. The most strikingwas an apparent complementary difference in predominant $alpha$ isoformsbetween dorsal and ventral horn. The parenchyma of dorsal hornstained most brightly for $alpha$ 1, whereas ventral horn stained mostbrightly for $alpha$ 3. The complementary difference also was observedfor axons in the dorsal columns. The dorsal one-half of the dorsalcolumn, the gracile fascicle that consists of ascending sensoryaxons, was enriched in $alpha$ 1, and the ventral one-half of the dorsalcolumn, a descending corticospinal tract, was enriched in $alpha$ 3 aswell as $alpha$ 1. These and the lateral $alpha$ 3-containing axon tracts arepresumably the origin of the unidentified $alpha$ 1- versus $alpha$ 3-containingmyelinated tracts observed previously in the rat medulla (McGrailet al., 1991). In addition, the endothelial cells that line thecentral canal were stained brightly for $alpha$ 1, but not for $alpha$ 2 or $alpha$ 3, whereas the ensheathing pial membranes and fragments of duramater stained for all three isoforms.

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Figure 3. Immunofluorescence detection of Na,K-ATPase isoforms in nontransgenic controls and transgenic mutant SOD1 mice. Tissue sections were labeled with monoclonal antibodies to $alpha$ 1 (6F), $alpha$ 2 (McB2), and $alpha$ 3 (XVIF9G10). Images were taken at 10×, and montages were made to display the entire section. D, Dorsal horn; G, gray matter; W, white matter; V, ventral horn; gf, gracile fascicle of ascending sensory axons; cs, corticospinal tract. The arrow points to the ependyma lining the central canal.

When they were compared with nontransgenic controls, there were markedly lower levels of staining for all three Na,K-ATPase $alpha$ isoforms in transgenic mutant SOD1 animals (Fig. 3). If lossesin Na,K-ATPase had been attributable to specific cell loss orto the atrophy of axons, the remaining cells would have more normalstain intensity. The uniformity of the loss of stain was the mostnotable feature, extending even to the ependymal lining of thecentral canal. The pial membranes, which appeared somewhat disruptedin the mutant mice, penetrated the white matter tracts more thanthey should, and their stain for $alpha$ 3 virtually wasabolished.

In contrast, and consistent with the immunoblots shown above, staining patterns for $beta$ 1 and $beta$ 2 subunits were unaltered in thetransgenic mutant SOD1 mice (Fig. 4). The principal differencethat was seen was in the diffusely shrunken appearance of thepathological spinal cord. A lack of effect on $beta$ expression suggestsa lack of effect on Na,K-ATPase expression and biosynthesis, asdiscussed below.

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Figure 4. Immunodetection of Na,K-ATPase $beta$ isoforms in nontransgenic controls and transgenic mutant SOD1 mice. Tissue sections were labeled with monoclonal antibodies to $beta$ 1 (BSP-3) and $beta$ 2 (426).

NO is unable to regulate Na,K-ATPase activity in spinal cord of transgenic mice

In some tissues NO is a normal Na,K-ATPase regulator acting through cGMP. Because free radical homeostasis appears to be perturbedin some forms of ALS, we tested whether regulation of the Na,K-ATPasewas affected in this model. Spinal cord tissue slices from nontransgeniccontrol mice were exposed to the NO donors SNP (Garthwaite etal., 1995) and DETA-NO (Diodati et al., 1993) for 15 min. Bothdonors caused a marked reduction (35-45%) of ouabain-sensitiveNa,K-ATPase activity (Fig. 5A). The effects were specific to Na,K-ATPase,because no measurable changes were observed in the ouabain-insensitive(Mg-ATPase) activity (data not shown). Many of the physiologicalactions of NO on Na,K-ATPase activity involve activation of solubleguanylate cyclase (McKee et al., 1994; Nathanson et al., 1995;Scavone et al., 1995; Ellis et al., 2000, 2001). When SNP- orDETA-NO-treated spinal cord tissue slices were exposed to ODQ,an inhibitor selective for soluble guanylate cyclase (Garthwaiteet al., 1995), it primarily blocked the SNP- and DETA-NO-inducedinhibition of ouabain-sensitive Na,K-ATPase activity (Fig. 5A).

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Figure 5. SNP- and DETA-NO-induced inhibition of ouabain-sensitive Na,K-ATPase was abolished in transgenic mutant SOD1 mice and transgenic normal human SOD1 overexpressors. Spinal cord tissue slices were incubated with or without ODQ (1 µM) for 3 min at 34°C, followed by incubation with DETA-NO (100 µM) or SNP (100 µM) for 15 min at 34°C. Drugs were removed, tissue slices were homogenized, and ouabain-sensitive Na,K-ATPase activity was measured. For all graphs that are shown, activity is expressed as µmol P_i/hr per milligram of protein, and values represent the means ± SEM for experiments on three animals done in triplicate. A, Ouabain-sensitive Na,K-ATPase activity in nontransgenic controls. *Significantly different from the control at p < 0.05 (by ANOVA and Fisher's PLSD). ^##Significantly different from DETA-NO- and SNP-treated samples at p < 0.05 (by ANOVA and Fisher's PLSD). B, C, Ouabain-sensitive Na,K-ATPase activity in transgenic mutant SOD1 and transgenic SOD1 normal human SOD1 overexpressors.

The effects of NO donors on activity in tissue slices from spinal cord of transgenic mutant SOD1 mice and of transgenic normalhuman SOD1 overexpressors are shown in Figure 5, B and C. Thebasal Na,K-ATPase activity was low, and neither SNP nor DETA-NOfurther inhibited it. The addition of ODQ in the presence of SNPor DETA-NO, or alone, failed to alter ouabain-sensitive Na,K-ATPaseactivity in spinal cord tissue slices of transgenic mutant SOD1mice (Fig. 5B) or transgenic normal human SOD1 overexpressors(Fig. 5C). Because ODQ treatment did not restore the lost activity,the data argue against a high basal level of otherwise-normalNO-mediated regulation as the cause of Na,K-ATPase inhibitionin the transgenic mice. These results indicate a surprisinglycomplete perturbation, in normal SOD1 overexpressors as well asmutants, of a regulatory pathway that in physiological conditionsdepends on the diffusion of NO from its site of synthesis to solubleguanylatecyclase.

The ability of NO donors to increase levels of cGMP by activating soluble guanylate cyclase was tested in the three groupsof mice. In nontransgenic control mice the addition of DETA-NOto spinal cord tissue slices caused a 40% increase in cGMP levelsthat, as expected, was abolished by the guanylate cyclase inhibitorODQ (Fig. 6A). In contrast, there were no measurable changes incGMP levels in either transgenic mutant SOD1 mice or transgenicnormal human SOD1 overexpressors treated with DETA-NO, ODQ, orDETA-NO plus ODQ (Fig. 6B,C). This could mean that soluble guanylatecyclase, like Na,K-ATPase, is inactivated in these mice, possiblytargeted by its specific binding site for a free radical, althoughsuch losses were not reported in the G1L strain of G93A mice,which expresses mutant SOD1 at a lower level (Facchinetti et al.,1999). Alternatively, the NO generated by the artificial donorscould be consumed rapidly in reactions catalyzed by the aberrantelevated levels of SOD1.

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Figure 6. cGMP levels are unaltered in transgenic SOD1 mice in response to DETA-NO treatment. Spinal cord tissue slices from nontransgenic controls (A), transgenic mutant SOD1 mice (B), or transgenic normal human SOD1 overexpressors (C) were incubated for 3 min at 34°C with ODQ (1 µM), followed by incubation for 15 min at 34°C with DETA-NO (100 µM). After centrifugation the supernatant was removed and assayed for cGMP, expressed as pmol/mg protein. *Significantly different from the control group at p < 0.05 (by ANOVA, Fisher's PLSD, and Scheffé's F test). Values for cGMP levels represent the means ± SEM for three experiments.

The pathway downstream of guanylate cyclase was tested by exposure of spinal cord tissue slices to the permeable protein kinaseG activator, 8-Br-cGMP. Figure 7A shows that in nontransgeniccontrols this caused an inhibition of Na,K-ATPase activity aseffective as DETA-NO treatment. However, there were no changesin activity in tissue from transgenic mutant SOD1 mice (Fig. 7B).Evidence for the involvement of protein phosphorylation in mediatingthe normal NO-induced regulation of Na,K-ATPase activity is shownin Figure 7 also. The addition of okadaic acid (400 nM) at concentrationsknown to inhibit protein phosphatases type 1 and type 2A mimickedthe effects of DETA-NO and 8-Br-cGMP in inhibiting ouabain-sensitiveNa,K-ATPase activity in nontransgenic SOD1 controls (Fig. 7A).Okadaic acid had no effect, however, on transgenic mutant SOD1mice (Fig. 7B). The inability to bypass any step of the NO-mediatedregulatory pathway is evidence either for the broadly compromisedstate of the transgenic spinal cord or for the resistance of theresidual Na,K-ATPase activity to any further regulation.

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Figure 7. Ouabain-sensitive Na⁺,K-ATPase activity in spinal cord of nontransgenic control mice (A) and transgenic mutant SOD1 mice (B) after incubation with DETA-NO (100 µM), 8-Br-cGMP (2 mM), or okadaic acid (OKA; 400 nM). Results are expressed as µmol P_i/hr per milligram of protein, and values represent the means ± SEM for three animals done in triplicate. *Significantly different from the control at p < 0.05 (by ANOVA and Fisher's PLSD).

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

The mechanisms of motor neuron death in ALS are unknown, but several theories have been proposed, including that mutationsin SOD1 may result in oxidative stress (Beckman et al., 1993;Crow et al., 1997; Andrus et al., 1998), increases in NO synthaseand reactivity of astrocytes (Almer et al., 1999), and glutamateexcitotoxicity secondary to glutamate transporter defects (Rothsteinet al., 1993; Bruijn et al., 1997; Trotti et al., 1999). Otherpossible causes of neuronal degeneration include alterations inmitochondrial function (Beal, 1995; Klivenyi et al., 1999), formationof mutant SOD1 protein aggregates (Bruijn et al., 1998), and improperassembly of intermediate filaments that have particular impacton motor neurons because of their exceptionally long axons (forreview, see Cleveland and Rothstein, 2001; Julien, 2001). Althoughall of these may contribute to the pathology and some may determinethe selective vulnerability of motor neurons, perturbation offree radical homeostasis directly related to the SOD1 mutationis the phenomenon that is least likely to be secondary to theneurodegeneration process. Curiously, selective expression ofmutant SOD1 in either astrocytes or neurons alone has failed toinduce the disease (Gong et al., 2000; Pramatarova et al., 2001;Lino et al., 2002).

Uniform loss of Na,K-ATPase

These studies demonstrate that there are surprisingly large decreases in ouabain-sensitive Na,K-ATPase in spinal cord of transgenicmutant SOD1 mice, as assessed by enzyme activity, $alpha$ subunit content,and anatomical distribution. Because of the uniformity, the lossesare not likely to be a secondary consequence of neuron atrophyor death; this was confirmed by the observation of similar lossesof Na,K-ATPase in the cerebellum. There were less severe decreasesin Na,K-ATPase in the mice overexpressing transgenic normal humanSOD1. SOD1 overexpression, which occurs in Down's syndrome asa direct result of trisomy, also is thought to increase oxidativedamage (Ceballos-Picot et al., 1991; Lee et al., 2001), exacerbateexcitotoxicity (Bar-Peled et al., 1996), and affect hippocampalultrastructure and function (Barkats et al., 1993; Gahtan et al.,1998). Because the transgenic normal human SOD1 mice we used donot show hallmarks of ALS pathology such as SOD1 aggregates, intermediatefilament aggregates, and mitochondrial defects, the observed Na,K-ATPaselosses are more likely to be attributable to a "gain of function"abnormality of free radical or oxidant homeostasis than to ALS-associatedneurodegeneration. These findings suggest that decreased Na,K-ATPaseactivity contributes to SOD1 ALS via inactivation and the lossof all three $alpha$ subunits.

Any given cell type expresses a particular combination of $alpha$ and $beta$ subunits (McGrail et al., 1991; Watts et al., 1991; Penget al., 1997; Wetzel et al., 1999; Martin-Vasallo et al., 2000).Many neurons, for example, express $alpha$ 3 $beta$ 1, mature astrocytes express $alpha$ 2 $beta$ 2, and oligodendrocytes express $alpha$ 2 $beta$ 3, but there are exceptions,such as the granule neurons of the cerebellum that express $alpha$ 3 $beta$ 2,Müller glial cells that express $alpha$ 1 $beta$ 2, and neurons that expressmore than one assembled complex. Decreases in $alpha$ 3 are diagnosticfor neuronal defects, because this isoform is not expressed inglia. Decreases in $alpha$ 2 are additional evidence that astrocytesas well as neurons are affected in the disease. Two well establishedfunctions of glia are the clearance of potassium and the Na⁺-dependent uptake of glutamate from the extracellular space aftersynaptic activation. Na,K-ATPase is activated when [Na⁺]_i rises concomitantly with glutamate uptake (Rose and Ransom,1996), and this stimulates the uptake of K⁺. The importance of these observations to ALS is highlighted byreports of selective loss of the astrocyte-specific glutamatetransporter EAAT2 (GLT-1) (Rothstein et al., 1995) and of itsvulnerability to oxidation by certain mutant SOD1 forms (Trottiet al., 1999). A defect in the glutamate transporter, a defectin the underlying glial sodium pump activity, and a defect inNa,K-ATPase activity in the neurons themselves are compatiblewith previous proposals that excitotoxicity contributes to theprogression ofALS.

Detection of the simultaneous loss of Na,K-ATPase $alpha$ isoforms specific to all different cell types in the spinal cord paintsa compelling picture of a defect that is not confined to the motorneurons that die, however. The implications of the diffuse natureof the Na,K-ATPase alterations are potentially far-reaching. Itsuggests, for one thing, that the mutant mice have a "sick cord"and that studies of almost any candidate protein could revealalterations that may contribute to the final pathology. It alsosuggests that alterations in the barrier organs such as the ependymaand pia may contribute to the disease. The loss of one-half tothree-quarters of the enzyme that is the largest consumer of ATPmay help to offset the effects of mitochondrial pathology andsuggests that further investigation of energy metabolism in ALSwould be fruitful (Browne et al., 1998; Klivenyi et al., 1999;Ames, 2000).

Altered free radical homeostasis and regulation of Na,K-ATPase

The NO/soluble guanylate cyclase pathway was altered severely in both transgenic mutant human SOD1 mice and transgenic normalhuman SOD1 overexpressors, whereas it inhibited ouabain-sensitiveNa,K-ATPase activity in nontransgenic control mice. NO-mediatedregulation of Na,K-ATPase activity is known in other tissues,including ciliary process and choroid plexus (Ellis et al., 2000,2001). In the CNS, NO modulates cerebral blood flow and synaptictransmission via the activation of soluble guanylate cyclase andincreases in cGMP (Murad, 1998). The loss of NO regulation intransgenic mutant SOD1 mice might have been predicted, consideringthe severity of the illness. However, the total blockade of theNO/cGMP pathway for Na,K-ATPase regulation in transgenic normalSOD1 overexpressors wasunexpected.

The role of NO in CNS-related diseases is not completely clear. Several lines of evidence have emerged that suggest that NOcan be either neuroprotective (Lipton et al., 1993; Chiueh, 1999)or neurodestructive (Dawson et al., 1991, 1992; Samdani et al.,1997). NO generated from NO donors or synthesized endogenouslyafter activation of the ionotropic glutamate receptor (Lafon-Cazalet al., 1993) can lead to neurotoxicity in part by reaction withsuperoxide anion and the subsequent formation of peroxynitrite(Lipton et al., 1993; Beckman and Koppenol, 1996). In contrast,other studies have demonstrated that the neuroprotective effectsof NO in CNS may result from nitration or nitrosylation of iron-or thiol-containing proteins (Stamler et al., 1992; Lipton etal., 1993; Chiueh, 1999). Such chemical modifications may altersignificantly the biological activity of the protein and minimizethe generation of reactive oxygen species and associated oxidativestress. A lack of effect on ALS pathology when G93A mice werecrossed with neuronal nitric oxide synthase (nNOS) knock-out micesuggested no involvement, but residual nNOS activity because ofthe synthesis of truncated forms complicated the interpretation(Facchinetti et al., 1999).

The degree of inhibition of Na,K-ATPase activity in transgenic mutant mice exceeded the decrease in the $alpha$ subunit. The Na,K-ATPasecan be inhibited chemically by oxygen free radicals and theirby-products (Mense et al., 1997). For example, superoxide anion,hydrogen peroxide, and hydroxyl radicals inhibited Na,K-ATPaseactivity, and this decrease correlated with increased lipid peroxidation(Viani et al., 1991; Huang et al., 1992). Of interest is the findingthat various NO donors (excluding sodium nitroprusside) causedsubstantial direct alterations in Na,K-ATPase activity via reactionwith free sulfhydryl groups (Boldyrev et al., 1997; Sato et al.,1997). Furthermore, as with other proteins (Stadtman, 1992), exposureof the Na,K-ATPase to free radicals made it more susceptible todegradation by proteolytic enzymes (Huang et al., 1992; Thevenodand Friedmann, 1999). Because $alpha$ and $beta$ subunits normally are foundin a 1:1 ratio, the reduction in $alpha$ , but not $beta$ , was unexpected.The data are consistent with greater vulnerability of the $alpha$ subunitto damage and degradation. This is plausible, considering thatthe majority of the mass of the $beta$ subunit is in the extracellularspace where it is adapted to a more oxidizing environment thanthe cytoplasm, and that its six extracellular sulfhydryl groupsare all in buried disulfide bonds. Most of the mass of the $alpha$ subunit,in contrast, is in the reducing environment on the cytoplasmicside of the membrane, and it has 23 free sulfhydryls and otheroxidizablegroups.

The widespread defects in Na,K-ATPase, not confined to either neurons or glia, support the original hypothesis that perturbationof free radical homeostasis is the most likely root cause of mutantSOD1 ALS pathology. The abrogation of the NO/cGMP pathway of Na,K-ATPaseregulation is an unexpected and potentially important event, whetherit is a parallel defect with the same root cause or a causativestep in Na,K-ATPaseloss.

  FOOTNOTES

Received June 27, 2002; revised Sept. 30, 2002; accepted Oct. 4, 2002.

This work was supported by grants from the Amyotrophic Lateral Sclerosis Association and the Fiftieth Anniversary ScholarsProgram of Harvard Medical School to D.Z.E. and by National Institutesof Health Grant R01-NS27653 to K.J.S. We thank Dr. Robert H. BrownJr. (Massachusetts General Hospital) for advice and stimulatingdiscussions. We are also grateful to Drs. J. Kyte, P. Martin-Vasallo,C. Goridis, and M. Schachner forantibodies.

Correspondence should be addressed to Dr. Kathleen J. Sweadner, 149-6118, Massachusetts General Hospital, 149 13th Street,Charlestown, MA 02129. E-mail: sweadner{at}helix.mgh.harvard.edu.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Almer G, Vukosavic S, Romero N, Przedborski S (1999) Inducible nitric oxide synthase up-regulation in a transgenic mouse model of familial amyotrophic lateral sclerosis. J Neurochem 72:2415-2425[ISI][Medline].
Ames III A (2000) CNS energy metabolism as related to function. Brain Res Brain Res Rev 34:42-68[Medline].
Andrus PK, Fleck TJ, Gurney ME, Hall ED (1998) Protein oxidative damage in a transgenic mouse model of familial amyotrophic lateral sclerosis. J Neurochem 71:2041-2048[ISI][Medline].
Barkats M, Bertholet J-Y, Venault P, Ceballos-Picot I, Nicole A, Phillips J, Moutier R, Roubertoux P, Sinet PM, Cohen-Salmon M (1993) Hippocampal mossy fiber changes in mice transgenic for the human copper/zinc superoxide dismutase gene. Neurosci Lett 160:24-28[Medline].
Bar-Peled O, Korkotian E, Segal M, Groner Y (1996) Constitutive overexpression of Cu/Zn superoxide dismutase exacerbates kainic acid-induced apoptosis of transgenic Cu/Zn superoxide dismutase neurons. Proc Natl Acad Sci USA 93:8530-8535[Abstract/Free Full Text].
Beal MF (1995) Aging, energy, and oxidative stress in neurodegenerative diseases. Ann Neurol 38:357-366[ISI][Medline].
Beckman JS, Koppenol WH (1996) Nitric oxide, superoxide, and peroxynitrite: the good, the bad, and the ugly. Am J Physiol 271:C1424-C1437[Abstract/Free Full Text].
Beckman JS, Carson M, Smith CD, Koppenol WH (1993) ALS, SOD, and peroxynitrite. Nature 364:584[Medline].
Blanco G, Mercer RW (1998) Isozymes of the Na-K-ATPase: heterogeneity in structure, diversity in function. Am J Physiol 275:F633-F650[Abstract/Free Full Text].
Boldyrev AA, Bulygina ER, Kramarenko GG, Vanin AF (1997) Effect of nitroso compounds on Na/K-ATPase. Biochim Biophys Acta 1321:243-251[Medline].
Brines ML, Robbins RJ (1992) Inhibition of $alpha$ 2/ $alpha$ 3 sodium pump isoforms potentiates glutamate neurotoxicity. Brain Res 591:94-102[ISI][Medline].
Brines ML, Dare AO, de Lanerolle NC (1995) The cardiac glycoside ouabain potentiates excitotoxic injury of adult neurons in rat hippocampus. Neurosci Lett 191:145-148[ISI][Medline].
Brown Jr RH (1995) Amyotrophic lateral sclerosis: recent insights from genetics and transgenic mice. Cell 80:687-692[ISI][Medline].
Browne SE, Bowling AC, Baik MJ, Gurney ME, Brown Jr RH, Beal MF (1998) Metabolic dysfunction in familial, but not sporadic, amyotrophic lateral sclerosis. J Neurochem 71:281-287[ISI][Medline].
Bruijn LI, Becher MW, Lee MK, Anderson KL, Jenkins NA, Copeland NG, Sisodia SS, Rothstein JD, Borchelt DR, Price DL, Cleveland DW (1997) ALS-linked SOD1 mutant G85R mediates damage to astrocytes and promotes rapidly progressive disease with SOD1-containing inclusions. Neuron 18:327-338[ISI][Medline].
Bruijn LI, Houseweart MK, Kato S, Anderson KL, Anderson SD, Ohama E, Reaume AG, Scott RW, Cleveland DW (1998) Aggregation and motor neuron toxicity of an ALS-linked SOD1 mutant independent from wild-type SOD1. Science 281:1851-1854[Abstract/Free Full Text].
Calabresi P, De Murtas M, Pisani A, Stefani A, Sancesario G, Mercuri NB, Bernardi G (1995) Vulnerability of medium spiny striatal neurons to glutamate: role of Na⁺/K⁺-ATPase. Eur J Neurosci 7:1674-1683[ISI][Medline].
Ceballos-Picot I, Nicole A, Briand P, Grimber G, Delacourte A, Defossez A, Javoy-Agid F, Lafon M, Blouin JL, Sinet PM (1991) Neuronal-specific expression of human copper/zinc superoxide dismutase gene in transgenic mice: animal model of gene dosage effects in Down's syndrome. Brain Res 552:198-214[ISI][Medline].
Chiueh CC (1999) Neuroprotective properties of nitric oxide. Ann NY Acad Sci 890:301-311[Abstract/Free Full Text].
Cleveland DW, Rothstein JD (2001) From Charcot to Lou Gehrig: deciphering selective motor neuron death in ALS. Nat Rev Neurosci 2:806-819[ISI][Medline].
Crambert G, Hasler U, Beggah AT, Yu C, Modyanov NN, Horisberger J-D, Lelievre L, Geering K (2000) Transport and pharmacological properties of nine different human Na,K-ATPase isozymes. J Biol Chem 275:1976-1986[Abstract/Free Full Text].
Crow JP, Sampson JB, Zhuang Y, Thompson JA, Beckman JS (1997) Decreased zinc affinity of amyotrophic lateral sclerosis-associated superoxide dismutase mutants leads to enhanced catalysis of tyrosine nitration of peroxynitrite. J Neurochem 69:1936-1944[ISI][Medline].
Dawson TM, Dawson VL, Snyder SH (1992) A novel neuronal messenger molecule in brain: the free radical, nitric oxide. Ann Neurol 32:297-311[ISI][Medline].
Dawson VL, Dawson TM, London ED, Bredt DS, Snyder SH (1991) Nitric oxide mediates glutamate neurotoxicity in primary cortical cultures. Proc Natl Acad Sci USA 88:6368-6371[Abstract/Free Full Text].
Diodati JG, Quyyumi AA, Keefer LK (1993) Complexes of nitric oxide with nucleophiles as agents for the controlled biological release of nitric oxide: hemodynamic effects in rabbit. J Cardiovasc Pharmacol 22:287-292[ISI][Medline].
Ellis DZ, Nathanson JA, Sweadner KJ (2000) Carbachol inhibits Na⁺-K⁺-ATPase activity in choroid plexus via stimulation of the NO/cGMP pathway. Am J Physiol 279:C1685-C1693[Abstract/Free Full Text].
Ellis DZ, Nathanson JA, Rabe J, Sweadner KJ (2001) Carbachol and NO inhibit Na,K-ATPase in ciliary process via activation of guanylate cyclase and cGMP. Invest Ophthalmol Vis Sci 42:2625-2631[Abstract/Free Full Text].
Facchinetti F, Sasaki M, Cutting FB, Zhai P, MacDonald JE, Reif D, Beal MF, Huang PL, Dawson TM, Gurney ME, Dawson VL (1999) Lack of involvement of neuronal nitric oxide synthase in the pathogenesis of a transgenic mouse model of familial amyotrophic lateral sclerosis. Neuroscience 90:1483-1492[ISI][Medline].
Gahtan E, Auerbach JM, Groner Y, Segal M (1998) Reversible impairment of long-term potentiation in transgenic Cu/Zn SOD mice. Eur J Neurosci 10:538-544[ISI][Medline].
Garthwaite J, Southam E, Boulton CL, Nielsen EB, Schmidt K, Mayer B (1995) Potent and selective inhibition of nitric oxide-sensitive guanylyl cyclase by ¹H-[1,2,4]oxadiazolo[4,3-a]quinoxalin-1-one. Mol Pharmacol 48:184-188[Abstract].
Gong YH, Parsadanian AS, Andreeva A, Snider WD, Elliott JL (2000) Restricted expression of G86R Cu/Zn superoxide dismutase in astrocytes results in astrocytosis but does not cause motoneuron degeneration. J Neurosci 20:660-665[Abstract/Free Full Text].
Gurney ME, Pu H, Chiu AY, Dal Canto MC, Polchow CY, Alexander DD, Caliendo J, Hentati A, Kwon YW, Deng H-X, Chen W, Zhai P, Sufit L, Siddique T (1994) Motor neuron degeneration in mice that express a human Cu/Zn superoxide dismutase mutation. Science 264:1772-1775[Abstract/Free Full Text].
Hieber V, Siegel GJ, Fink DJ, Beaty MW, Mata M (1991) Differential distribution of (Na,K)-ATPase $alpha$ isoforms in the central nervous system. Cell Mol Neurobiol 11:253-262[ISI][Medline].
Huang WH, Wang Y, Askari A (1992) (Na⁺ + K⁺)-ATPase: inactivation and degradation induced by oxygen radicals. Int J Biochem 24:621-626[ISI][Medline].
Julien J-P (2001) Amyotrophic lateral sclerosis: unfolding the toxicity of the misfolded. Cell 104:581-591[ISI][Medline].
Kim MS, Akera T (1987) O₂ free radicals: cause of ischemia-reperfusion injury to cardiac Na⁺,K⁺-ATPase. Am J Physiol 252:H252-H257[Abstract/Free Full Text].
Klivenyi P, Ferrante RJ, Matthews RT, Bogdanov MB, Klein AM, Andreassen OA, Mueller G, Wermer M, Kaddurah-Daowk R, Beal MF (1999) Neuroprotective effects of creatine in a transgenic animal model of amyotrophic lateral sclerosis. Nat Med 3:347-350.
Lafon-Cazal M, Pietri S, Culcasi M, Bockaert J (1993) NMDA-dependent superoxide production and neurotoxicity. Nature 364:535-537[Medline].
Lee M, Hyun D-H, Jenner P, Halliwill B (2001) Effect of overexpression of wild-type and mutant Cu/Zn superoxide dismutases on oxidative damage and antioxidant defenses: relevance to Down's syndrome and familial amyotrophic lateral sclerosis. J Neurochem 76:957-965[ISI][Medline].
Lees GJ, Leong W (1996) Interactions between excitotoxins and the Na⁺,K⁺-ATPase inhibitor ouabain in causing neuronal lesions in the rat hippocampus. Brain Res 714:145-155[Medline].
Lees GJ, Lehmann A, Sandberg M, Hamberger A (1990) The neurotoxicity of ouabain, a sodium/potassium ATPase inhibitor, in the rat hippocampus. Neurosci Lett 120:159-162[ISI][Medline].
Lino MM, Schneider C, Caroni P (2002) Accumulation of SOD1 mutants in postnatal motoneurons does not cause motoneuron pathology or motoneuron disease. J Neurosci 22:4825-4832[Abstract/Free Full Text].
Lipton SA, Choi Y-B, Pan Z-H, Lei SZ, Chen H-S, Sucher NJ, Loscalzo J, Singel DJ, Stamler JS (1993) A redox-based mechanism for the neuroprotective and neurodestructive effects of nitric oxide and related nitroso compounds. Nature 364:626-632[Medline].
Martin-Vasallo P, Wetzel RK, Garcia-Segura LM, Molina-Holgado E, Arystarkhova E, Sweadner KJ (2000) Oligodendrocytes in brain and optic nerve express the $beta$ 3 subunit isoform of Na,K-ATPase. Glia 31:206-218[ISI][Medline].
Mata M, Siegel GJ, Hieber V, Beaty MW, Fink DJ (1991) Differential distribution of (Na,K)-ATPase $alpha$ isoform mRNAs in the peripheral nervous system. Brain Res 546:47-54[ISI][Medline].
McGrail KM, Phillips JM, Sweadner KJ (1991) Immunofluorescent localization of three Na,K-ATPase isozymes in the rat central nervous system: both neurons and glia can express more than one Na,K-ATPase. J Neurosci 11:381-391[Abstract].
McKee M, Scavone C, Nathanson JA (1994) Nitric oxide, cGMP, and hormone regulation of active sodium transport. Proc Natl Acad Sci USA 91:12056-12060[Abstract/Free Full Text].
McLean IW, Nakane PK (1974) Periodate-lysine-paraformaldehyde fixative. A new fixative for immunoelectron microscopy. J Histochem Cytochem 22:1077-1083[Abstract].
Mense M, Stark G, Apell H-J (1997) Effects of free radicals on partial reactions of the Na,K-ATPase. J Membr Biol 156:63-71[ISI][Medline].
Murad F (1998) Nitric oxide signaling: would you believe that a simple free radical could be a second messenger, autacoid, paracrine substance, neurotransmitter, and hormone? Recent Prog Horm Res 53:43-59.
Nathanson JA, Scavone C, Scanlon C, McKee M (1995) The cellular Na⁺ pump as a site of action for carbon monoxide and glutamate: a mechanism for long-term modulation of cellular activity. Neuron 14:781-794[ISI][Medline].
Peng L, Martin-Vasallo P, Sweadner KJ (1997) Isoforms of Na,K-ATPase $alpha$ and $beta$ subunits in the rat cerebellum and in granule cell cultures. J Neurosci 17:3488-3502[Abstract/Free Full Text].
Pramatarova A, Laganiere J, Roussel J, Brisebois K, Rouleau GA (2001) Neuron-specific expression of mutant superoxide dismutase 1 in transgenic mice does not lead to motor impairment. J Neurosci 21:3369-3374[Abstract/Free Full Text].
Rose CR, Ransom BR (1996) Mechanisms of H⁺ and Na⁺ changes induced by glutamate, kainate, and D-aspartate in rat hippocampal astrocytes. J Neurosci 16:5393-5404[Abstract/Free Full Text].
Rosen DR, Siddique T, Patterson D, Figlewicz DA, Sapp P, Hentati A, Donaldson D, Goto J, O'Regan JP, Deng HX, Gusella JS, Horvitz HR, Brown Jr RH (1993) Mutations in Cu/Zn superoxide dismutase gene are associated with familial amyotrophic lateral sclerosis. Nature 362:59-62[Medline].
Rothstein JD, Jin L, Dykes-Hoberg M, Kuncl RW (1993) Chronic inhibition of glutamate uptake produces a model of slow neurotoxicity. Proc Natl Acad Sci USA 90:6591-6595[Abstract/Free Full Text].
Rothstein JD, Van Kammen M, Levey AI, Martin LJ, Kuncl RW (1995) Selective loss of glial glutamate transporter GLT-1 in amyotrophic lateral sclerosis. Ann Neurol 38:73-84[ISI][Medline].
Samdani AF, Newcamp C, Resink A, Facchinetti F, Hoffman BE, Dawson VL, Dawson TM (1997) Differential susceptibility to neurotoxicity mediated by neurotrophins and neuronal nitric oxide synthase. J Neurosci 17:4633-4641[Abstract/Free Full Text].
Sato T, Kamata Y, Irifune M, Nishikawa T (1997) Inhibitory effect of several nitric oxide-generating compounds on purified Na,K-ATPase activity from porcine cerebral cortex. J Neurochem 68:1312-1318[ISI][Medline].
Scavone C, Scanlon C, McKee M, Nathanson JA (1995) Atrial natriuretic peptide modulates sodium and potassium-activated adenosine triphosphatase through a mechanism involving cyclic GMP and cyclic GMP-dependent protein kinase. J Pharmacol Exp Ther 272:1036-1043[Abstract/Free Full Text].
Stadtman ER (1992) Protein oxidation and aging. Science 257:1220-1224[Abstract/Free Full Text].
Stamler JS, Singel DJ, Loscalzo J (1992) Biochemistry of nitric oxide and its redox-activated forms. Science 258:1898-1902[Abstract/Free Full Text].
Stelmashook EV, Weih M, Zorov D, Vicotrov I, Dirnagl U, Isaev N (1999) Short-term block of Na⁺/K⁺-ATPase in neuro-glial cell cultures of cerebellum induces glutamate-dependent damage of granule cells. FEBS Lett 456:41-44[Medline].
Sweadner KJ (1989) Isozymes of the Na⁺/K⁺-ATPase. Biochim Biophys Acta 988:185-220