Disease Progression in a Transgenic Model of Familial Amyotrophic Lateral Sclerosis Is Dependent on Both Neuronal and Non-Neuronal Zinc Binding Proteins

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

A correction has been published

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (38)

Citing Articles via Google Scholar

Google Scholar

Articles by Puttaparthi, K.

Articles by Elliott, J. L.

Search for Related Content

PubMed

PubMed Citation

Articles by Puttaparthi, K.

Articles by Elliott, J. L.

Previous Article  |  Next Article

The Journal of Neuroscience, October 15, 2002, 22(20):8790-8796

Disease Progression in a Transgenic Model of Familial Amyotrophic Lateral Sclerosis Is Dependent on Both Neuronal and Non-Neuronal Zinc Binding Proteins
Krishna Puttaparthi¹, William L. Gitomer², Uma Krishnan¹, Marjatta Son¹, Bhagya Rajendran¹, and Jeffrey L. Elliott¹
Departments of ¹ Neurology and ² Internal Medicine, University of Texas, Southwestern Medical Center, Dallas, Texas 75390

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mutations in the Cu/Zn superoxide dismutase (SOD1) gene cause one form of familial amyotrophic lateral sclerosis, a progressivedisorder of motor neurons leading to weakness and death of affectedindividuals. Experiments using both transgenic mice expressingmutant SOD1 and SOD1 knock-out mice have demonstrated that diseaseis caused by a toxic gain of function and not by a loss of normalSOD1 activity. Precise mechanisms underlying mutant SOD1 toxicityare unclear but may involve abnormal interactions between zincandSOD1.
The metallothioneins (MTs) represent a family of zinc binding proteins that can function as zinc chaperones for apo-SOD1 invitro. We hypothesized that manipulation of metallothioneins invivo might alter the disease phenotype of transgenic mice expressingG93A SOD1 and therefore crossed this line with MT-I and MT-IIor MT-III knock-out mice. G93A SOD1 mice deficient of either MT-Iand MT-II or MT-III exhibited significant reductions in survivalcompared with G93A SOD1 mice. In addition, motor dysfunction wasmarkedly accelerated in G93A SOD1 mice deficient in metallothioneinswith regard to onset (MT-I and MT-II) or progression (MT-III).
These results indicate that the disease course in G93A SOD1 mice is dependent on levels of metallothionein expression. BecauseMT-I and MT-II are expressed in glia whereas MT-III is found inneurons, these results also indicate that primary changes withinnon-neuronal cells can affect mutant SOD1-induced disease anddo so in ways distinct from primary neuronalchanges.

Key words: amyotrophic lateral sclerosis; metallothionein; copper; zinc; glia; transgenic

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although mechanisms underlying mutant superoxide dismutase (SOD1) toxicity remain unclear, abnormalities in zinc binding toSOD1 have been implicated in disease pathogenesis (Elliott, 2001).Zinc is important in maintaining the structural integrity of SOD1,and, when depleted of zinc, SOD1 gains enhanced ability to reactwith peroxynitrite and catalyze the addition of nitro groups totyrosine residues (Lyons et al., 1996; Crow et al., 1997a; Gotoet al., 2000). Mutant SOD1 exhibits markedly reduced affinityfor zinc compared with wild-type SOD1 and has enhanced nitrationactivity (Crow et al., 1997a,b). Indeed, biochemical hallmarksof protein nitration, including elevated 3-nitrotyrosine products,have been found in spinal cords from amyotrophic lateral sclerosis(ALS) patients and mutant SOD1 (mSOD1) transgenic mice (Beal etal., 1997; Bruijn et al., 1997a; Ferrante et al., 1997; Toghiet al., 1999). Zinc binding may also be important in modulatingprotein aggregation, another possible mechanism of toxicity (Johnstonet al., 2000; Cherney et al., 2001; Curtain et al., 2001; Quaglioet al., 2001). Recent work has addressed biological consequencesof zinc-depleted SOD1, finding that it is highly toxic when introducedinto motor neurons in vitro (Estevez et al., 1999). However, experimentsdirectly assessing the role of zinc in disease pathogenesis havebeen limited, partly because of the difficulty in altering zincbinding in live animals. To address the role of zinc in mSOD1toxicity in vivo, we used an alternative approach involving themanipulation of proteins involved in zinc homeostasis with subsequentanalysis of changes in diseasephenotype.

The metallothioneins (MTs) represent a family of zinc binding proteins, three of which, MT-I, MT-II, and MT-III, are foundin the murine nervous system. Metallothioneins are important inthe regulation of zinc bioavailability within cells, by actingas chaperones during the synthesis of metalloenzymes (Jacob etal., 1998; Palmiter, 1998). Metallothioneins are rich in cysteineresidues that bind zinc and can be readily oxidized with subsequentrelease of zinc to accepting proteins, including apo-SOD1 (Suzukiand Kuroda, 1995). Experiments using genetically altered micewith metallothionein overexpression or deletions have shown thatthese proteins protect the CNS from oxidative injury or heavymetal toxicity (Masters et al., 1994b; Erickson et al., 1997).Metallothionein expression is markedly upregulated in the spinalcords of ALS patients and transgenic mutant SOD1 mice, suggestingthat these molecules also serve a protective function in diseasepotentially related to their zinc binding capacity (Smitt et al.,1992; Blaauwgeers et al., 1996; Gong and Elliott, 2000). Therefore,we decided to use changes in metallothionein expression to studythe role of zinc in mutant SOD1 toxicity in vivo. Consequently,we crossed transgenic mice expressing a G93A SOD1 mutation withMT-I and MT-II or MT-III knock-out mice and then studied changesin the diseasephenotype.

Motor neuron dysfunction and degeneration are hallmarks of ALS, but recent work using tissue-specific expression of mutantSOD1 in transgenic mice has suggested that interactions betweenneurons and glia may be necessary to generate a disease phenotype(Gong et al., 2000; Pramatarova et al., 2001). The differentialexpression of metallothioneins within the CNS can also be usedto assess potential neuronal and glial contributions to the diseaseprocess. Because MT-I and MT-II are restricted to glia whereasMT-III is neuronal, targeted manipulation of distinct metallothioneinsallows change within each cellular compartment (glial or neuronal)to be made directly and independently (Nishimura et al., 1992;Palmiter et al., 1992; Masters et al., 1994a; Gong and Elliott,2000). Our results indicate that both neuronal and non-neuronalcells contribute to disease progression in G93A SOD1mice.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mouse lines, breeding strategy, and genotyping. Transgenic mice expressing the low copy number human G93A SOD1 mutation (B6SJL-TgNSOD1-G93A;JR2300) were obtained from The Jackson Laboratory (Bar Harbor,ME). Mice with targeted deletions of both MT-I and MT-II loci(129S7/SvImJ) were also obtained from The Jackson Laboratory.MT-III knock-out mice (129Sv/C5Bl) were generously provided byDr. Richard Palmiter (University of Washington, Seattle, WA) andhave been well characterized (Erickson et al., 1997). Two differingbreeding paradigms were used for MT-I and MT-II or MT-III crossingwith G93A SOD1 transgenic mice. For an accelerated breeding program(B_a), G93A SOD1 mice were crossed to either MT-I and MT-II orMT-III knock-out mice. F1 offspring, all heterozygous for metallothioneinexpression and G93A SOD1 positive, were then backcrossed to metallothioneinhomozygous founders. Progeny, heterozygous for metallothioneinand G93A SOD1 positive, were then bred with metallothionein heterozygoussiblings. This cross allows all possible genotypes to be generatedwith adequate internal controls, and consequently only these micewere included in the study. A prolonged breeding paradigm (B_p)was also used for crossing G93A SOD1 mice with MT-I and MT-IIknock-out mice. Using this strategy, G93A SOD1 transgenic micewere crossed with MT-I and MT-II knock-out mice. F1 offspringwere then backcrossed for eight generations onto the G93A SOD1strain. After the eighth generation, metallothionein heterozygotespositive for G93A SOD1 were then bred to metallothionein heterozygoussiblings, again allowing all potential genotypes to be generatedandanalyzed.

Offspring were genotyped using genomic DNA isolated from tails digested overnight with proteinase K at 50°C. The followingprimer pairs for PCR were used: 5'-CAT CAG CCC TAA TCC ATC TGA-3'and 5'-CGC GAC TAA CAA TCA AAG TGA-3'. This will amplify a 236bp fragment from mice carrying the human G93A SOD1 transgenicconstruct. 5'- CGC GCT CAC TGA CTG CCT TC-3' and 5'-CTG GGAGCAGCA CTT CGC ACA GC-3' will amplify a 282 and 299 bp fragment fromwild-type or MT-II knock-out alleles, respectively. 5'-ACG TAGCGC ATC CGC TTG-3' and 5'-CTC TTC TTG CAG TTC GTG C-3' will amplifya 154 bp fragment from a wild-type MT-III allele. 5'-CTT GGG TGGAGA GGC TAT TC-3' and 5'-AGG TGA GAT GAC AGG AGA TC-3' will amplifya 280 bp fragment from the neomycin cassette used to generatethe MT-III knock-out.

Motor testing and survival analysis. The stride test was performed with slight modifications from previously published methods(Gong et al., 2000). Mice had their hindpaws dipped in nontoxicink and were trained to walk across the 1 m white board for recordingfootprints. Stride lengths were measured in millimeters. Miceunable to move hindlimbs and perform this task were graded aszero. Statistical analysis was performed using the Student's ttest. Forelimb grip testing was done with a grip metertransducer(Ugo Basile, Comerio, Italy) designed especially for mouse. Atmonthly testing intervals, three independent trials were performed,with the top two being averaged. Animals unable to grip were recordedas zero. All procedures performed on mice were approved by ananimal research committee (ARC, University of Texas, SouthwesternMedical Center, Dallas, TX) and conform to National Institutesof Health guidelines. Animals unable to correct posture when placedon side were considered end stage and killed. Survival analysiswas performed using the Kaplan-Meiermethod.

Immunochemistry and histology. After overdose with pentobarbital (250 mg/kg, i.p.), animals were killed and then perfusedwith 4% paraformaldehyde for spinal cord and brain removal. Forimmunohistochemistry, paraffin-embedded sections (10 µm) wereincubated with a rabbit polyclonal GFAP antibody (1:250 dilution;Dako, High Wycombe, UK), visualized using an immunoperoxidasereaction (the one kit; Sternberger Monoclonals, Lutherville, MD),and counterstained with cresyl violet (.5%). For motor neuroncounting, 8 µm sections of L5-L6 spinal cord from paraffin-embeddedtissue were stained with 0.5% cresyl violet. Random sections throughthe L5-L6 cord were selected and used for counting. Motor neuronswere identified using established criteria (Deckwerth et al.,1996; Reaume et al., 1996; Kostic et al., 1997), and the numberof motor neurons per spinal cord section was counted by an examinerunaware of the animal genotype. At least five sections per animalwere used, and the average number of motor neurons per slice peranimal wasassessed.

Western blotting. Animals were overdosed with sodium pentobarbital (250 mg/kg, i.p.). Spinal cords were dissected and homogenizedin 20 mM Tris-HCl, pH 7.5, 2 mM DTT, 0.1 mg of leupeptin, 1 mMEDTA, and 1 mM EGTA. The homogenate was then centrifuged at 14,000× g to pellet debris. Protein concentration was measured usingthe BCA protein assay (Pierce, Rockford, IL). Protein (25 µg)from each sample was run on a 4-20% Tris-glycine gel (Invitrogen,San Diego, CA). After transfer, membranes were washed in PBS,followed by overnight incubation in blocking buffer [0.2% I-block(Applied Biosystems, Foster City, CA), PBS, and 0.1% Tween 20].The membrane was then probed with a polyclonal rabbit anti-bovineSOD1 (Chemicon, Temecula, CA) antibody at 1:4000 dilution. Afterseveral washes, membranes were incubated with an alkaline phosphatase-conjugatedsecondary antibody (1:5000 in blocking buffer), and the immunoreactivesignals were visualized using an enhanced chemiluminescent reagent,CDP Star (Western Star kit; Tropix). After exposure, films werescanned and then imported into NIH Image for quantitation of banddensity.

Zinc determination. Mice from 5.5-6 months of age were used for zinc determination. Mice were overdosed with sodium pentobarbital(250 mg) and perfused with PBS before tissue removal. All glasswarewas first soaked in 5% nitric acid and then rinsed with 18 M $Omega$ deionized water before use. Animal tissue was hydrolyzed overnightin 70% "ultraspec" nitric acid at 102°C. Sample blanks, consistingof nitric acid only heated overnight, were included with tissuesamples. Total zinc was determined using a Varian Spectra AA-20atomic spectrophotometer at 213.9 nm wavelength according to theinstructions of the manufacturer. Three to four animals were usedper group. Units for zinc are given in micrograms per gram ofwet weight oftissue.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Expression of glial metallothioneins influences survival and disease course in G93A SOD1 transgenic mice

To assess a potential role for glial metallothioneins (MT-I and MT-II) in mutant SOD1-induced disease, we crossed G93A SOD1transgenic mice with knock-out mice lacking both MT-I and MT-II.These double knock-out mice have a normal lifespan and do notexhibit a motor neuron phenotype. Initially, we used an acceleratedbreeding program (rapid backcross to metallothionein strain) togenerate and compare G93A SOD1 mice with the three possible metallothioneingenotypes (wild type, heterozygous, and homozygous knock-outs).The survival curves for the accelerated paradigm are shown inFigure 1. G93A SOD1 mice deficient in MT-I and MT-II demonstrateda significantly reduced mean survival (204 ± 4 d) compared withG93A SOD1 mice with normal metallothionein expression (240 ± 3d; p < 0.0001). This 36 d change corresponds to a 15% overallreduction in G93A SOD1 lifespan. G93A SOD1 mice heterozygous forMT-I and MT-II also exhibited a significant reduction in meansurvival (221 ± 4 d), although not to the same degree as homozygousknock-outs. Thus, survival in G93A SOD1 mice is dependent on MT-Iand MT-II expression in a dose-dependent manner. These resultssuggest that primary changes within non-neuronal cell populationscan significantly affect survival of mutant SOD1 mice.

View larger version (22K):
[in this window]
[in a new window]
Figure 1. Kaplan-Meier cumulative survival analysis of G93A SOD1 mice with or without MT-I and MT-II expression following the accelerated breeding protocol. Survival in G93A SOD1 mice is dependent on levels of MT-I and MT-II expression (log-rank test; p < 0.0001). MT $-$ / $-$ , MT-I and MT-II knock-outs; MT+/ $-$ , mice heterozygous for both MT-I and MT-II.

To ensure that survival changes observed in G93A SOD1 mice lacking MT-I and MT-II were not attributable to artifacts of crossbreeding, we repeated the experiment using a prolonged breedingprotocol that sought to place the mice on the original G93A transgenicbackground. The results are shown in Figure 2A. G93A SOD1 micedeficient in MT-I and MT-II had a significantly reduced mean survival(229 ± 5 d) compared with G93A SOD1 mice with normal metallothioneinexpression (261 ± 4 d; p < 0.0001). This 32 d change correspondsto a 12% reduction in overall G93A SOD1 lifespan. As in the acceleratedbreeding paradigm, G93A SOD1 mice heterozygous for MT-I and MT-IIdemonstrated a reduction in survival of significant but intermediateproportions (249 ± 4 d). Thus, results obtained from two varyingbreeding protocols demonstrate a similar dose-dependent effectof MT-I and MT-II expression on the survival of G93A SOD1 mice.

View larger version (22K):
[in this window]
[in a new window]
Figure 2. Survival and onset of motor dysfunction is influenced by levels of MT-I and MT-II expression (prolonged breeding protocol). A, Kaplan-Meier cumulative survival analysis (log-rank test; p < 0.0001). B, Stride length analysis; onset of motor dysfunction is significantly influenced by non-neuronal metallothionein expression levels. C, Grip strength analysis; onset of motor dysfunction is significantly affected by non-neuronal metallothionein expression. MT $-$ / $-$ , MT-I and MT-II knock-outs; MT+/ $-$ , mice heterozygous for both MT-I and MT-II.

We also performed longitudinal analysis of motor function using both stride length and grip strength to determine the effectsof MT-I and MT-II expression on disease onset and progression.Measurement of stride length is primarily an indicator of hindlimbmotor function and has been well characterized in mutant SOD1transgenic mice (Gong et al., 2000). By 6 months of age, G93ASOD1 mice have begun to develop abnormalities in gait characterizedby stride shortening, which then progress over the next 2 monthsat a rate of 1.2 cm/month (Fig. 2B). In contrast, G93A SOD1 micedeficient for MT-I and MT-II demonstrated onset of gait abnormalitiesat a much earlier age. A decrease in stride length was apparentin these mice between 3 and 4 months of age and thereafter continuedto decline at a rate of 0.7 cm/month. G93A SOD1 mice heterozygousfor MT-I and MT-II demonstrated onset of abnormal gait at 5 monthsof age, again intermediate between G93A SOD1 and metallothionein-deficientG93A SOD1 mice. We then used grip strength as a primary measureof forelimb motor function in these mice (Fig. 2C). G93A SOD1mice demonstrated onset of significant grip weakness between 6and 7 months of age. However, the onset of grip weakness was significantlyaccelerated in G93A SOD1 mice lacking both MT-I and MT-II, withinitial declines observed between 4 and 5 months of age. Again,G93A SOD1 mice heterozygous for the MT-I and MT-II allele firstexhibited grip weakness at an intermediate time point between5 and 6months.

Results from these tests of motor function reveal a dose-dependent effect of MT-I and MT-II on the course of motor dysfunctionin G93A SOD1 similar to what was observed for survival. However,although survival was shifted by ~1 month in G93A SOD1 mice lackingboth MT-I and MT-II, the onset of motor dysfunction was shiftedeven more robustly. Thus, changes in non-neuronal metallothioneinexpression appear to alter the onset of motor dysfunction in mutantSOD1 mice to a greater extent than overallsurvival.

We next investigated whether G93A SOD1 deficient in MT-I and MT-II demonstrated any changes in spinal cord pathology to accompanythe observed alterations in motor function. Spinal cords fromendstage G93A SOD1 mice (8.5 months) and G93A SOD1 mice lackingMT-I and MT-II (7.5 months) showed extensive astrogliosis andmicrogliosis throughout the spinal cord and brainstem. Both linesalso demonstrated significant and comparable neuronal dropout,with an ~75% loss in lumbar ventral horn motor neurons. The pathologyin presymptomatic (3 month) G93A SOD1 mice and G93A SOD1 micelacking MT-I and MT-II demonstrated mild astroglial changes andneuronal loss. Examination of tissue from an early symptomatictime point (5.25 months) indicated enhanced astroglial changesin the spinal cords of G93A SOD mice lacking MT-I and MT-II comparedwith G93A SOD1 mice with normal MT-I and MT-II (Fig. 3A,B). Inaddition, increased GFAP reactivity was observed in white mattertracts of spinal cord and brainstem compared with tissue fromage-matched G93A SOD1 mice (Fig. 3C,D). However, despite differencesin non-neuronal pathology and motor deficits, neuronal loss inthe lumbar ventral horn was similar in G93A SOD1 mice with orwithout MT-I and MT-II at each examined time point, includingpresymptomatic, early symptomatic, and end stage (Fig. 4). Theseresults indicate that, even if motor neurons are present, theymay be dysfunctional and therefore cause a decline in motor function.

View larger version (158K):
[in this window]
[in a new window]
Figure 3. GFAP immunoreactivity is increased in G93A SOD1 mice lacking MT-I and MT-II. A, B, L5-L6 spinal cord ventral horn from 5.25-month-old G93A SOD1 transgenic mice with normal MT-I and MT-II (A) or absent MT-I and MT-II (B). C, D, Cerebellar white matter from 5.25-month-old G93A SOD1 transgenic mice with normal MT-I and MT-II (C) or absent MT-I and MT-II (D). Magnification, 200×. Arrowheads, GFAP reactive cells.

View larger version (43K):
[in this window]
[in a new window]
Figure 4. Motor neuron counts performed on L5-L6 spinal cords at various functional time points. Motor neuron survival in G93A SOD1 mice is not affected by levels of non-neuronal metallothionein (MT-I and MT-II) expression. n = 4 for each group.

Survival in G93A SOD1 mice is dependent on neuronal MT-III expression

To address whether altering zinc binding proteins in neurons might also influence the course of mSOD1-induced disease in vivo,we crossed G93A SOD1 transgenic mice with MT-III knock-out mice.Because previous experiments using MT-I and MT-II knock-out micedid not demonstrate significant differences between the acceleratedand prolonged breeding paradigms, we selected the acceleratedbreeding paradigm for generating G93A SOD1 mice lacking MT-III.

The effects of reducing MT-III expression on the survival of G93A SOD1 mice are shown in Figure 5. MT-III knock-out mice lackingthe G93A SOD1 mutation do not exhibit any change in motor functionor survival compared with wild-type mice. G93A SOD1 mice deficientfor both MT-III alleles demonstrate a marked reduction in overallsurvival compared with G93A SOD1 mice possessing both wild-typeMT-III alleles. The mean survival for G93A SOD1 mice (253 ± 6d) was reduced by over 20% to 202 ± 4 d (p < 0.0001 log-rank test)for G93A SOD1 mice lacking both MT-III alleles. No significantchange in survival was observed for G93A SOD1 mice heterozygousfor MT-III (249 ± 6 d), indicating that one MT-III allele is sufficientto rescue the original phenotype and contrasts to the dose-dependentsurvival effects described previously for the non-neuronal metallothioneins.

View larger version (30K):
[in this window]
[in a new window]
Figure 5. Survival and disease course is influenced by MT-III expression. A, Kaplan-Meier cumulative survival analysis (log-rank test; p < 0.0001). B, Stride length analysis; progression but not onset of motor dysfunction is significantly affected by neuronal MT-III expression. C, Grip strength analysis; progression of motor dysfunction is significantly affected by neuronal MT-III expression. MT $-$ / $-$ , MT-III knock-outs; MT+/ $-$ , mice heterozygous for MT-III.

If survival in G93A SOD1 mice lacking MT-III is shortened by almost 2 months, we then asked whether a corresponding temporalshift in motor function also occurred in these mice. Longitudinalassessment of stride length in G93A SOD1 mice lacking MT-III revealedsignificant differences in motor function compared with G93A SOD1mice (Fig. 5B). Although both groups displayed a similar onsetof gait abnormality between 5 and 6 months of age, the declinein motor function was much steeper for G93A SOD1 mice lackingMT-III (2 cm) than for G93A SOD1 mice (1.2 cm). Similar changeswere observed for grip strength (Fig. 5C). G93A SOD1 mice withand without MT-III exhibit normal grip strength until 5 monthsof age. After this time point, G93A SOD1 mice lacking MT-III showan accelerated rate of decline in motor function compared withG93A SOD1 mice. Thus, MT-III expression within neurons greatlyaffects survival of G93A SOD1 mice and markedly influences progressionof mutant SOD1-induceddisease.

Pathologic examination of spinal cord from presymptomatic and end stage G93A SOD1 mice with or without MT-III expression didnot reveal significant differences in neuronal survival. However,at an early symptomatic time point (5.25 months), G93A mice lackingMT-III exhibited a significant increase in motor neuron loss comparedwith G93A mice with normal MT-III levels (Fig. 6). Thus, in micewith alterations in neuronal MT-III, the increased severity ofmotor dysfunction parallels the more pronounced loss of motorneurons observed. This pattern is in contrast to the knock-outof non-neuronal metallothioneins in which the more severe changesin motor function are not matched by a more significant loss ofmotor neuron number.

View larger version (87K):
[in this window]
[in a new window]
Figure 6. Motor neuron loss is enhanced in G93A SOD1 mice lacking MT-III. A, L5-L6 ventral horn from a 5.25-month-old G93A SOD1 transgenic mouse with normal MT-III. B, L5-L6 ventral horn from a 5.25-month-old G93A SOD1 transgenic mouse lacking MT-III. Magnification, 400×. C, Motor neuron counts performed on L5-L6 spinal cords at various functional time points. Motor neuron survival in G93A SOD1 mice is affected by levels of neuronal MT-III expression at an early symptomatic time point. *p < 0.03. n = 4 for each group.

Because of the importance of metallothioneins in zinc homeostasis, we next asked whether altering MT-III expression withinthe CNS of G93A SOD1 mice in fact led to corresponding changesin zinc levels. Total zinc levels in brain were determined foradult wild-type, MT-III knock-out, and G93A SOD1 mice with normaland absent MT-III expression. Zinc levels in MT-III knock-outmice were significantly lower than in wild-type mice (11.7 ± 0.1vs 13.0 ± 0.1 µg/gm tissue; p < 0.01). Zinc levels in G93A SOD1mice (18.6 ± 1.0 µg/gm tissue; p < 0.002) were significantly higher(>50%) than in wild-type mice. G93A SOD1 mice lacking any MT-IIIexpression also demonstrated significantly increased zinc levels(16.8 ± 0.2 µg/gm tissue; p < 0.004) compared with wild-type mice,although not to the same degree as G93A SOD1 mice with normalMT-III expression. Zinc levels in the brains of G93A SOD1 micelacking MT-III were reduced compared with G93A SOD1 mice withnormal MT-III expression, although results did not reach significance(p < 0.07) because of variance in G93A SOD1 values. These resultsindicate that the total zinc pool within the CNS is reduced inmice lacking MT-III, raising the possibility that less zinc maybe available for binding toSOD1.

Changes in disease phenotype are not related to increases in mutant SOD1 protein expression

Because the severity of mutant SOD1-induced disease in transgenic mice, both in terms of onset and progression, is clearlydependent on levels of mutant SOD1, we wanted to determine whetheraltering metallothionein synthesis could in fact result in changesof SOD1 protein expression. Western blot analysis of spinal cordand liver extracts from adult G93A SOD1 mice and from G93A SOD1mice deficient in either MT-III or MT-I and MT-II show equivalentlevels of mutant SOD1 protein expression (Fig. 7). Thus, the changesin disease phenotype manifested in the absence of metallothioneinexpression are not simply attributable to a compensatory increasein mutant SOD1 protein levels.

View larger version (43K):
[in this window]
[in a new window]
Figure 7. Western blot of adult mouse spinal cord and liver probed with SOD1 antibody. hSOD1, Human SOD1; mSOD1, normal murine SOD1. Spinal cord extract (25 µg) and 15 µg of liver extract were loaded per lane.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Precise mechanisms underlying mutant SOD1 toxicity in ALS remain unclear, but there is growing evidence to support a potentialrole for zinc in the disease process. The mutations in SOD1 linkedto familial ALS (FALS) span all five exons of the coding regionand encompass virtually all functional domains of the protein,including the copper binding site, active site, dimer interface,and $beta$ structural regions (Gaudette et al., 2000). However, toour knowledge, no mutations in the four zinc binding residuesin SOD1 have been identified in FALS, suggesting that interactionsbetween zinc and SOD1 may be important for disease expression.Although zinc binding sites may be preserved in SOD1 mutationscausing disease, studies have shown that zinc binding to mutantSOD1 is abnormal with consequences both for the enzymatic andstructural integrity of the protein. Abnormal zinc binding toSOD1 results in its increased ability to catalyze addition ofnitro groups to protein tyrosine residues. Changes in zinc bindingalso enhance the tendency of certain proteins, including prionprotein and $beta$ amyloid, to form insoluble complexes, and such mechanismsmay contribute to the formation of SOD1 aggregates observed inthe disease (Johnston et al., 2000; Cherney et al., 2001; Curtainet al., 2001; Quaglio et al., 2001). Our findings that diseaseprogression in G93A SOD1 transgenic mice is markedly affectedby the expression of zinc binding metallothioneins provide onemore piece of evidence to implicate interactions of zinc withmutant SOD1 as a contributing factor to the diseasephenotype.

There are a number of ways in which changes in metallothionein expression might promote mutant SOD1-induced toxicity. Metallothioneinscan function as zinc chaperones, ferrying zinc ions to certainapo-proteins, and in vitro experiments have found that metallothioneinscan perform this function for apo-SOD1 (Suzuki and Kuroda, 1995).Without metallothioneins, it may be harder to ensure adequatezinc loading for apo-SOD1, particularly in the context of thedecreased affinity for zinc manifested by mutant SOD1 comparedwith wild-type SOD1 (Crow et al., 1997a). Our findings indicatingoverall lower zinc levels in mice deficient for MT-III would beconsistent with this hypothesis. Experiments have demonstratedthat zinc-deficient SOD1 is highly toxic to motor neurons in culture,and similar processes may also occur in vivo (Estevez et al.,1999). Metallothioneins also buffer excess zinc and protect cellsfrom the potentially harmful consequences of excessive intracellularzinc. SOD1 is normally expressed at high levels within the CNS,comprising 1% of total protein, and, with up to a 20-fold decreasein zinc affinity for mutant SOD1 compared with wild-type SOD1,conditions may favor release of zinc from mutant SOD1 (Crow etal., 1997a; Elliott, 2001). Excess zinc may be toxic through avariety of pathways, including modulation of glutamate receptoror transporter function, thus leaving neurons vulnerable to excitotoxicity(Sensi et al., 1999; Trotti et al., 1999; Mitrovic et al., 2001).Recent work has suggested that, at least in yeast, SOD1 itselfmay play an important role in zinc metabolism (Wei et al., 2001).

It is also possible that the protective effects of metallothioneins in G93A SOD1 mice may be unrelated to specific interactionswith SOD1 but rather act through indirect and nonspecific mechanisms.Metallothioneins clearly protect cells against oxidative injuryin general and may perform similar roles in mutant SOD1-induceddisease. Recently, experiments have demonstrated that metallothioneinsmay also be found in mitochondria and appear to be important inmodulating cellular respiration via changes in zinc levels withinmitochondria (Ye et al., 2001). The absence of metallothioneinscould potentially lead to abnormal cellular respiration and enhancedmitochondrial dysfunction in cells already subjected to mutantSOD1 toxicity. In fact, studies from mutant SOD1 transgenic miceindicate that early and prominent mitochondrial pathology is ahallmark of mutant SOD1-induced disease (Dal Canto and Gurney,1994; Wong et al., 1995). Recent evidence suggests that some SOD1may also localize to mitochondria, allowing for direct interactionsbetween metallothionein and SOD1 in this organelle (Okado-Matsumotoand Fridovich, 2001; Sturtz et al., 2001).

Neuronal and non-neuronal cells in mutant SOD1-induced disease

The restricted expression of distinct metallothioneins in either glia or neurons also allows an assessment of both neuronaland non-neuronal contributions to the disease process. Althoughmotor neuron dysfunction and degeneration are hallmarks of ALS,recent work has demonstrated that mutant SOD1 expression restrictedto neurons is not sufficient to cause weakness in transgenic mice,suggesting that expression of mutant SOD1 in other cell typesis necessary for the disease phenotype (Pramatarova et al., 2001).Glia cells, particularly astrocytes, may contribute to the generationof disease. Astrocytes develop early pathologic features, includingSOD1-positive aggregate formation and selective loss of the principalglutamate transporter EAAT-2 (excitatory amino acid transporter-2)with concomitant alterations in glutamate transport function (Rothsteinet al., 1995; Bruijn et al., 1997b; Canton et al., 1998). Indeed,expression of mSOD1 can result in a post-translational inactivationof this glutamate transporter, potentially leading to the increasesin extracellular glutamate observed both in familial ALS patientsand mSOD1 transgenic mice (Rothstein et al., 1992; Trotti et al.,1999: Alexander et al., 2000). However, targeted expression ofmutant SOD1 in astrocytes in transgenic mice, although resultingin astrocytosis, does not cause a motor phenotype or neuronalloss (Gong et al., 2000). Thus, experiments using cell-specificexpression of mutant SOD1 suggest that defects in both neuronaland non-neuronal cells may be necessary for diseasemanifestation.

Our experimental results with metallothioneins indicate that both non-neuronal and neuronal dysfunction contribute to diseaseprogression and survival in this murine model of ALS but do soin disparate ways. Deletion of non-neuronal metallothioneins reducessurvival in G93A SOD1 mice by ~1 month but has a more marked effecton onset of motor deficits. However, this accelerated motor phenotypeoccurs without significant change in motor neuron number, indicatingthat extent of motor dysfunction and motor neuron loss may bediscordant. In contrast, removal of neuronal MT-III produces amarked change in survival and disease course that is congruentwith enhanced neuronal loss. Mechanisms underlying metallothionein-inducedchanges in either neuronal or non-neuronal populations from mutantSOD1 transgenic mice remain unclear but do not appear to be relatedto changes in mutant SOD1 expression. We are exploring currentlywhether those possible mechanisms include an enhanced capacityof SOD1 to catalyze peroxynitrite formation or an increased tendencyfor mutant SOD1 to form aggregates in the absence of metallothioneinexpression.

  FOOTNOTES

Received Feb. 19, 2002; revised June 25, 2002; accepted June 27, 2002.

This work was supported by National Institute of Neurological Disorders and Stroke Grant NS40911, the Muscular Dystrophy Association,and the Amyotrophic Lateral Sclerosis Association. We thank Dr.Richard Palmiter for the MT-III knock-out mice. We thank ChristineElliott, Yongli Kong, and Jill Marshall for expert technicalassistance.

Correspondence should be addressed to Dr. Jeffrey L. Elliott, Department of Neurology, University of Texas, Southwestern MedicalCenter, 5323 Harry Hines Boulevard, Dallas, TX 75390. E-mail:jellio{at}mednet.swmed.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alexander GM, Deitch JS, Seeburger JL, Del Valle L, Heiman-Paterson TD (2000) Elevated cortical extracellular glutamate in transgenic mice expressing mutant (G93A) Cu/Zn superoxide dismutase. J Neurochem 74:1666-1673[Medline].
Beal MF, Ferrante RJ, Browne SE, Mattews RT, Kowall NW, Brown Jr RH (1997) Increased 3-nitrotyrosine in both sporadic and familial amyotrophic lateral sclerosis. Ann Neurol 42:646-654.
Blaauwgeers HGT, Chand MA, van den Berg FM, Vianney de Jong JMB, Troost D (1996) Expression of different metallothionein messenger ribonucleic acids in motor cortex, spinal cord and liver from patients with amyotrophic lateral sclerosis. J Neurol Sci 142:39-44[Medline].
Bruijn LI, Beal MF, Becher MW, Schulz JB, Wong PC, Price DL, Cleveland DW (1997a) Elevated free nitrotyrsoine levels but not protein bound or hydroxyl radicals, throughout amyotrophic lateral sclerosis (ALS)-like disease implicate tyrosine nitration as an aberrant in vivo property of one familial ALS-linked superoxide dismutase 1 mutant. Proc Natl Acad Sci USA 94:7606-7611[Abstract/Free Full Text].
Bruijn LI, Becher MW, Lee MK, Anderson KL, Jenkins NA, Copeland NG, Sisodia SS, Rothstein JD, Borchelt DR, Price DL, Cleveland DW (1997b) ALS-linked SOD1 mutant G85R mediates damage to astrocytes and promotes rapidly progressive disease with SOD1-containing inclusions. Neuron 18:327-338[ISI][Medline].
Canton T, Pratt J, Stutzmann JM, Boireau A (1998) Glutamate uptake is decreased tardively in the spinal cord of FALS mice. NeuroReport 9:775-778[Medline].
Cherney RA, Atwood CS, Xilinas ME, Gray DN, Jones WD, McLean CA, Barnham KJ, Volitakis I, Fraser FW, Kim YS, Huang X, Goldstein LE, Moir RD, Lim JT, Beyreuther K, Zheng H, Tanzi RE, Masters CL, Bush AI (2001) Treatment with a copper-zinc chelator markedly and rapidly inhibits $beta$ -amyloid accumulation in Alzheimer's disease transgenic mice. Neuron 30:665-676[ISI][Medline].
Crow JP, Sampson JB, Zhuang Y, Thompson JA, Beckman JS (1997a) Decreased zinc affinity of amyotrophic lateral sclerosis-associated superoxide dismutase mutants leads to enhanced catalysis of tyrosine nitration by peroxynitrite. J Neurochem 69:1936-1944[ISI][Medline].
Crow JP, Ye YZ, Strong M, Kirk M, Barnes S, Beckman JS (1997b) Superoxide catalyzes nitration of tyrosines by peroxynitrite in the rod and head domains of neurofilament-L. J Neurochem 69:1945-1954[ISI][Medline].
Curtain CC, Ali F, Volitakis I, Cherney RA, Norton RS, Beyreuther K, Barrow CJ, Masters CL, Bush AI, Barnham KJ (2001) Alzheimer's disease amyloid- $beta$ binds to copper and zinc to generate an allosterically ordered membrane penetrating structure containing superoxide dismutase-like subunits. J Biol Chem 276:20466-20473[Abstract/Free Full Text].
Dal Canto MC, Gurney ME (1994) Development of central nervous system pathology in a murine transgenic model of ALS. Am J Pathol 145:1271-1280[Abstract].
Deckwerth TL, Elliott JL, Knudson CM, Johnson EM, Snider WD, Korsmeyer SJ (1996) Bax is required for neuronal death after trophic factor deprivation and during development. Neuron 17:401-411[ISI][Medline].
Elliott JL (2001) Zinc and copper in the pathogenesis of amyotrophic lateral sclerosis. Prog Neuropsychopharmacol Biol Psychiatry 25:1169-1185[Medline].
Erickson JC, Hollopeter G, Thomas SA, Froelick GJ, Palmiter RD (1997) Disruption of the metallothionein-III gene in mice: analysis of brain zinc, behavior, and neuron vulnerability to metals, aging, and seizures. J Neurosci 17:1271-1281[Abstract/Free Full Text].
Estevez AG, Crow JP, Sampson JB, Reiter C, Zhuang Y, Richardson GJ, Tarpey MM, Barbeito L, Beckman JS (1999) Induction of nitric oxide dependent apoptosis in motor neurons by zinc deficient superoxide dismutase. Science 286:2497-2500.
Ferrante RJ, Shinobu LA, Schulz JB, Mattews RT, Thomas CE, Kowall NW, Gurney ME, Beal MF (1997) Increased 3-nitrotyrosine and oxidative damage in mice with human copper/zinc superoxide dismutase mutation. Ann Neurol 42:326-334[ISI][Medline].
Gaudette M, Hirano M, Siddique T (2000) Current status of SOD1 mutations in familial amyotrophic lateral sclerosis. Amyotroph Lateral Scler Other Motor Neuron Disord 1:83-89[ISI][Medline].
Gong YH, Elliott JL (2000) Metallothionein expression is altered in a transgenic model of familial amyotrophic lateral sclerosis. Exp Neurol 162:735-742.
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].
Goto JJ, Zhu H, Sanchez RJ, Nersissian A, Gralla EB, Valentine JS (2000) Loss of in vitro metal binding in mutant copper-zinc superoxide dismutases associated with familial amyotrophic lateral sclerosis. J Biol Chem 275:1007-1014[Abstract/Free Full Text].
Jacob C, Maret W, Vallee BL (1998) Control of zinc transfer between thionein, metallothionein and zinc proteins. Proc Natl Acad Sci USA 95:3489-3494[Abstract/Free Full Text].
Johnston JA, Dalton MJ, Gurney ME, Kopito RR (2000) Formation of high molecular weight complexes of mutant Cu, Zn-superoxide dismutase in a mouse model for familial amyotrophic lateral sclerosis. Proc Natl Acad Sci USA 97:12571-12576[Abstract/Free Full Text].
Kostic V, Jackson-Lewis V, deBilbao F, Dubois-Dauphin M, Przedborski S (1997) Bcl-2: prolonging life in a transgenic mouse model of familial amyotrophic lateral sclerosis. Science 277:559-562[Abstract/Free Full Text].
Lyons TJ, Liu H, Goto JJ, Nersissian A, Roe JA, Graden JA, Cafe C, Ellerby LM, Bredesen DE, Gralla EB, Valentine JS (1996) Mutations in the copper-zinc superoxide dismutase that cause amyotrophic lateral sclerosis alter the zinc binding site and the redox behavior of the protein. Proc Natl Acad Sci USA 93:12240-12244[Abstract/Free Full Text].
Masters BA, Quaife CJ, Erickson JC, Kelly EJ, Froelick GJ, Zambrowicz BP, Brinster RL, Palmiter RD (1994a) Metallothionein III is expressed in neurons that sequester zinc in synaptic vesicles. J Neurosci 14:5844-5857[Abstract].
Masters BA, Kellly EJ, Quaife CJ, Brinster RL, Palmiter RD (1994b) Targeted disruption of metallothionein I and II genes increases sensitivity to cadmium. Proc Natl Acad Sci USA 91:584-588[Abstract/Free Full Text].
Mitrovic AD, Plesko F, Vandenberg RJ (2001) Zn²⁺ inhibits the anion conductance of the glutamate transporter EAAT4. J Biol Chem 276:26071-26076[Abstract/Free Full Text].
Nishimura N, Nishimura H, Ghaffar A, Tohyama C (1992) Localization of metallothionein in the brain of rat and mouse. J Histochem Cytochem 40:309-315[Abstract].
Okado-Matsumoto A, Fridovich I (2001) Subcellular localization of superoxide dismutases (SOD) in rat liver. J Biol Chem 276:38388-38393[Abstract/Free Full Text].
Palmiter RD (1998) The elusive function of metallothioneins. Proc Natl Acad Sci USA 95:8428-8430[Abstract/Free Full Text].
Palmiter RD, Findley SD, Whitmore TE, Durnham DM (1992) MT-III, a brain-specific member of the metallothionein gene family. Proc Natl Acad Sci USA 89:6333-6337[Abstract/Free Full Text].
Pramatarova A, Laganiere L, 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].
Quaglio E, Chiesa R, Harris DA (2001) Copper converts the cellular prion protein into a protease resistant species that is distinct from the scrapie isoform. J Biol Chem 276:11432-11438[Abstract/Free Full Text].
Reaume AG, Elliott JL, Hoffman EK, Kowall NW, Ferrante RJ, Siwek DF, Wilcox HM, Flood DG, Beal MF, Brown RH, Scott RW, Snider WD (1996) Motor neurons in Cu/Zn superoxide dismutase deficient mice develop normally but exhibit enhanced cell death after axonal injury. Nat Genet 13:43-47[ISI][Medline].
Rothstein JD, Martin LJ, Kuncl RW (1992) Decreased glutamate transport by the brain and spinal cord in amyotrophic lateral sclerosis. N Engl J Med 326:1464-1468[Abstract].
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].
Sensi SL, Yin HG, Carriedo SG, Rao SS, Weiss JH (1999) Preferentialz N²⁺ influx through Ca²⁺ permeable AMPA channels triggers prolonged mitochondrial superoxide production. Proc Natl Acad Sci USA 96:2414-2419[Abstract/Free Full Text].
Smitt PAE, Blaauwgeers HGT, Troost D, de Jong JMBV (1992) Metallothionein immunoreactivity is increased in the spinal cord of patients with amyotrophic lateral sclerosis. Neurosci Lett 144:107-110[ISI][Medline].
Sturtz LA, Diekert K, Jensen LT, Lill R, Culotta VC (2001) A fraction of yeast Cu, Zn superoxide dismutase and its metallochaperone, CCS, localize to the intermembrane space of mitochondria. J Biol Chem 276:38084-38089[Abstract/Free Full Text].
Suzuki T, Kuroda T (1995) Transfer of copper and zinc from ionic and metallothionein bound forms to Cu, Zn superoxide dismutase. Res Commun Mol Pathol Pharmacol 87:287-296[ISI][Medline].
Toghi H, Abe T, Yamazaki K, Murata T, Ishizaki E, Isobe C (1999) Remarkable increase in cerebrospinal fluid 3-nitrotyrosine in patients with sporadic amyotrophic lateral sclerosis. Ann Neurol 46:129-131[ISI][Medline].
Trotti D, Rolfs A, Danbolt NC, Brown Jr RH, Hediger MA (1999) SOD1 mutants linked to amyotrophic lateral sclerosis selectively inactivate a glial glutamate transporter. Nat Neurosci 2:427-433[ISI][Medline].
Wei JJ, Srinivasan C, Han H, Valentine JS, Gralla EB (2001) Evidence for a novel role for copper-zinc superoxide dismutase in zinc metabolism. J Biol Chem 276:44798-44803[Abstract/Free Full Text].
Wong PC, Pardo CA, Borchelt DR, Lee MK, Copeland NG, Jenkins NA, Sisodia SS, Cleveland DW, Price DL (1995) An adverse property of a familial ALS-linked SOD1 mutation causes motor neuron disease characterized by vacuolar degeneration of mitochondria. Neuron 14:1105-1116[ISI][Medline].
Ye B, Maret W, Vallee BL (2001) Zinc metallothionein imported into liver mitochondria modulates respiration. Proc Natl Acad Sci USA 98:2317-2322[Abstract/Free Full Text].

Copyright © 2002 Society for Neuroscience 0270-6474/02/22208790-07$05.00/0

This article has been cited by other articles:

R. S. Chung, M. Penkowa, J. Dittmann, C. E. King, C. Bartlett, J. W. Asmussen, J. Hidalgo, J. Carrasco, Y. K. J. Leung, A. K. Walker, et al.
Redefining the Role of Metallothionein within the Injured Brain: EXTRACELLULAR METALLOTHIONEINS PLAY AN IMPORTANT ROLE IN THE ASTROCYTE-NEURON RESPONSE TO INJURY
J. Biol. Chem., May 30, 2008; 283(22): 15349 - 15358.
[Abstract] [Full Text] [PDF]

M. Son, S. C. Leary, N. Romain, F. Pierrel, D. R. Winge, R. G. Haller, and J. L. Elliott
Isolated Cytochrome c Oxidase Deficiency in G93A SOD1 Mice Overexpressing CCS Protein
J. Biol. Chem., May 2, 2008; 283(18): 12267 - 12275.
[Abstract] [Full Text] [PDF]

J.-L. Gonzalez de Aguilar, C. Niederhauser-Wiederkehr, B. Halter, M. De Tapia, F. Di Scala, P. Demougin, L. Dupuis, M. Primig, V. Meininger, and J.-P. Loeffler
Gene profiling of skeletal muscle in an amyotrophic lateral sclerosis mouse model
Physiol Genomics, January 17, 2008; 32(2): 207 - 218.
[Abstract] [Full Text] [PDF]

C. Lai, X. Lin, J. Chandran, H. Shim, W.-J. Yang, and H. Cai
The G59S Mutation in p150glued Causes Dysfunction of Dynactin in Mice
J. Neurosci., December 19, 2007; 27(51): 13982 - 13990.
[Abstract] [Full Text] [PDF]

M. Son, K. Puttaparthi, H. Kawamata, B. Rajendran, P. J. Boyer, G. Manfredi, and J. L. Elliott
Overexpression of CCS in G93A-SOD1 mice leads to accelerated neurological deficits with severe mitochondrial pathology
PNAS, April 3, 2007; 104(14): 6072 - 6077.
[Abstract] [Full Text] [PDF]

J. Hidalgo, M. Penkowa, C. Espejo, E. M. Martinez-Caceres, J. Carrasco, A. Quintana, A. Molinero, S. Florit, M. Giralt, and A. Ortega-Aznar
Expression of Metallothionein-I, -II, and -III in Alzheimer Disease and Animal Models of Neuroinflammation.
Experimental Biology and Medicine, October 1, 2006; 231(9): 1450 - 1458.
[Abstract] [Full Text] [PDF]

Y. Zhang, H. Wang, J. Li, D. A. Jimenez, E. S. Levitan, E. Aizenman, and P. A. Rosenberg
Peroxynitrite-Induced Neuronal Apoptosis Is Mediated by Intracellular Zinc Release and 12-Lipoxygenase Activation
J. Neurosci., November 24, 2004; 24(47): 10616 - 10627.
[Abstract] [Full Text] [PDF]

H. G. Jeong, C.-K. Youn, H.-J. Cho, S.-H. Kim, M.-H. Kim, H.-B. Kim, I.-Y. Chang, Y.-S. Lee, M.-H. Chung, and H. J. You
Metallothionein-III Prevents {gamma}-Ray-induced 8-Oxoguanine Accumulation in Normal and hOGG1-depleted Cells
J. Biol. Chem., August 13, 2004; 279(33): 34138 - 34149.
[Abstract] [Full Text] [PDF]

M. Son, C. D. Cloyd, J. D. Rothstein, B. Rajendran, and J. L. Elliott
Aggregate Formation in Cu,Zn Superoxide Dismutase-related Proteins
J. Biol. Chem., April 11, 2003; 278(16): 14331 - 14336.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

A correction has been published

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager