DNA Methyltransferase Contributes to Delayed Ischemic Brain Injury

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The Journal of Neuroscience, May 1, 2000, 20(9):3175-3181

DNA Methyltransferase Contributes to Delayed Ischemic Brain Injury
Matthias Endres¹^,², Andreas Meisel², Detlev Biniszkiewicz³, Shobu Namura¹, Konstantin Prass², Karsten Ruscher², Andreas Lipski², Rudolf Jaenisch³, Michael A. Moskowitz¹, and Ulrich Dirnagl²
¹ Stroke and Neurovascular Regulation Laboratory, Massachusetts General Hospital, Harvard Medical School, Charlestown, Massachusetts 02129, ² Division of Experimental Neurology, Department of Neurology, Charite Hospital, 10098 Berlin, Germany, and ³ Whitehead Institute for Biomedical Research, Massachusetts Institute of Technology, Cambridge, Massachusetts 02142

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

DNA methylation is important for controlling the profile of gene expression and is catalyzed by DNA methyltransferase (MTase),an enzyme that is abundant in brain. Because significant DNA damageand alterations in gene expression develop as a consequence ofcerebral ischemia, we measured MTase activity in vitro and DNAmethylation in vivo after mild focal brain ischemia. After 30min middle cerebral artery occlusion (MCAo) and reperfusion, MTasecatalytic activity and the 190 kDa band on immunoblot did notchange over time. However, [³H]methyl-group incorporation into DNA increased significantlyin wild-type mice after reperfusion, but not in mutant mice heterozygousfor a DNA methyltransferase gene deletion (Dnmt^S/+). Dnmt^S/+ mice were resistant to mild ischemic damage, suggesting thatincreased DNA methylation is associated with augmented brain injuryafter MCA occlusion. Consistent with this formulation, treatmentwith the MTase inhibitor 5-aza-2'-deoxycytidine and the deacetylationinhibitor trichostatin A conferred stroke protection in wild-typemice. In contrast to mild stroke, however, DNA methylation wasnot enhanced, and reduced dnmt gene expression was not protectivein an ischemia model of excitotoxic/necrotic cell death. In conclusion,our results demonstrate that MTase activity contributes to poortissue outcome after mild ischemic braininjury.

Key words: cerebral ischemia; delayed cell death; DNA damage; DNA methylation; DNA methyltransferase; gene expression

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mammalian DNA methylation is a covalent, postreplicative modification of genomic DNA and has been implicated in developmentand differentiation (Li et al., 1992; Panning and Jaenisch, 1998),X-chromosome inactivation (Cedar and Razin, 1990), imprinting(Li et al., 1993; Razin and Cedar, 1994; Tucker et al., 1996a,b;Surani, 1998), and cancer (Baylin et al., 1991; Counts and Goodman,1995; Laird et al., 1995; Jones, 1996). DNA methylation is catalyzedby the maintenance DNA (cytosine-5) methyltransferase enzyme (MTase,EC 2.1.1.37) and S-adenosyl methionine (SAM) as methyl donor(Jones, 1996; Lengauer et al., 1997; Okano et al., 1998). Theprimary substrates for MTase are CpG dinucleotides, which representonly 1-2% of the total genome, and ~70-80% of all CpG sites aremethylated in adult somatic mammalian cells (Cross and Bird, 1995).Generally, DNA methylation represses gene transcription ("genesilencing"), whereas hypomethylation is correlated with activetranscription (Ehrlich and Wang, 1981; Adams and Burdon, 1982;Doerfler, 1983; Cedar, 1988; Bestor, 1990; Bird, 1992; Leonhardand Bestor, 1993; Laird and Jaenisch, 1996).

It is not known whether DNA methylation is important in ischemic brain damage, but it may be of particular interest in thiscontext because (1) MTase activity is unexpectedly high in neurons,implying a neuron-specific function in these nonreplicating cells(Goto et al., 1993; Brooks et al., 1996). (2) Brain ischemia causesDNA damage including G-T mismatches generated by deamination of5-methyl cytosine (5-MeC), a powerful endogenous mutagen; MTasemay therefore remethylate newly incorporated cytosines after DNArepair in brain (Brooks et al., 1996; Liu et al., 1996; MacManusand Linnik, 1997; Cui et al., 1999). In addition, the formationof 8-hydroxyguanine by oxygen radical injury during ischemia/reperfusionmay alter methylation of adjacent cytosines (Cerda and Weitzman,1997). (3) DNA methylation could alter gene expression, althoughit has not been determined whether changes in DNA methylationdevelop after cerebralischemia.

In this study we examined whether there are significant differences in MTase protein, enzyme activity, and DNA methylationafter experimental brain ischemia in mice and determined whetherreduced levels of MTase are associated with differences in strokeoutcome in transgenic mice heterozygous for a dnmt1 gene deletion(Dnmt^S/+mice).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Transgenic mice. Mice heterozygous for the maintenance DNA methyltransferase gene (Dnmt^S/+) were generated as described (Li et al., 1992, 1993). Dnmt^S/+ mice are healthy, fertile, and phenotypically normal; dnmt1 nullmice (Dnmt^S/S) die during embyronic development (Li et al., 1992, 1993). Allexperiments were performed using littermates (Dnmt^S/+ and Dnmt^+/+) in a pure 129/SV_Jaebackground.

Mouse model for focal cerebral ischemia. Animal experiments were performed according to National Institutes of Health andinstitutional guidelines and the policy on the use of animalsin neuroscience research of the Society for Neuroscience. Mice(18-22 gm) were anesthetized with 1.5% halothane (induction) andmaintained on 1.0% halothane in 70% N₂O and 30% O₂ by face mask.Focal cerebral ischemia was induced as described (Endres et al.,1998b). In brief, MCA occlusion was produced by a silicone-coated8-0 monofilament into the internal carotid artery. Thirty minutesor 2 hr later, the filament was withdrawn to reperfuse the brain.To insure equivalent levels of ischemia between groups, regionalcerebral blood flow (rCBF) was measured by laser Doppler flowmetryusing a flexible skull probe (Huang et al., 1994; Endres et al.,1998a). In randomly selected animals the left femoral artery wascannulated for arterial blood pressure and blood gas determination(Huang et al., 1994; Endres et al., 1998a). Arterial blood samples(50 µl) were analyzed for pH, partial pressure of oxygen (PaO₂)and partial pressure of carbon dioxide (PaCO₂) using a blood gas/pHanalyzer (Corning 178, Ciba-Corning Diagnostics, Medford, MA).Core temperature was maintained at ~37 ± 0.5°C with a thermostat(FHC, Brunswick, ME) and a heating lamp during the monitoringperiod until 1 hr afterreperfusion.

Western blotting. MTase protein levels were determined by immunoblots of extracts of olfactory bulb, striatum, and hippocampusin Dnmt^S/+ and Dnmt ^+/+ mice. To examine for time-dependent changes in MTase protein,129/SV_EvTacBr wild-type mice (Taconic Farms, Germantown, NY) underwent30 min MCAo as above followed by reperfusion (1-72 hr) (Endreset al., 1998b). After mice were killed, brains were immediatelyremoved. Ischemic tissue was identified using a dissecting microscope,and ischemic tissue only (mostly striatum) was isolated alongwith corresponding tissue from the contralateral side, snap-frozenin liquid nitrogen, and stored at $-$ 80°C until further use. Proteinswere isolated according to standard techniques, separated by a7% SDS/PAGE gel, and transferred onto a nitrocellulose membrane.Subsequently, blots were incubated with rabbit polyclonal antiserumHM334 (1:2000 dilution) that recognizes the following polypeptidesequence within mouse maintenance DNA methyltransferase: CRSPRSRPKPRGPRRSK(Tucker et al., 1996a). Bound protein was detected by chemiluminescence(ECL, Amersham Pharmacia Biotech, Piscataway, NJ). Coomassie bluestaining was performed to insure equivalent levels of proteinloading.

MTase catalytic activity assay. Animals underwent 30 min MCAo/reperfusion as above. Cortical and striatal tissue from eachhemisphere and cerebellum were separated, snap-frozen in liquidnitrogen, and stored at $-$ 80°C. Nuclear extracts were analyzedfor MTase activity as described (Li et al., 1992). Nuclear extract(5 µg) was incubated with 20 mM Tris-HCl, pH 7.4, 10 mM EDTA,10% glycerol, 2 mM DTT, 200 µM PMSF, 0.5 µM [³H]-SAM, 15 µg/ml RNase A, and 50 pmol hemimethylated oligo-probednMT1m2 (see below) in a total volume of 50 µl. The reaction wasinitiated by addition of nuclear extract and incubated for 1 hrat 37°C. Fifty microliters of 16 µM SAM were then added, and the[³H]dnMT1m2-probe was extracted with phenol/chloroform. Probes wereapplied to a positively charged Porablot plus membrane (pore size0.45 µm; Macherey-Nagel, Düren, Germany) using a dot blot apparatusand washed three times with 300 µl sterile H₂O. Membranes wereair-dried, and the respective areas were counted in 2 ml nonliquidscintillation solution (OptiPhase "Hi-Safe" II) using a scintillationcounter (LKB, EG&G Wallac, Gaithersburg, MD). MTase activity waslinear over time and enzyme dependent (data not shown). The oligodeoxynucleotideduplex probe dnMT1m2 was as follows: 5'-GAXGXGATCXGGTTAAXGAGTCXGATGXGTAG-3',3'-CTGCGCTAGGCCAATTGCTCAGGCTACGCATC-5'; X = 5-MeC.

In vivo DNA methylation assay. Two hundred microliters of PBS, pH 7.4, and 200 µl of [methyl-³H]methionine (200 µCi, specific activity 513 mCi/mg; AmershamLife Science, Freiburg, Germany) were continuously infused over2 hr via PE-10 interarterial catheter after 30 min MCA occlusion.Anesthesia was then stopped, and animals were placed in a cagefor an additional 10 hr before they were killed. Cortex, striatum,and cerebellum were removed and prepared as described above andsnap-frozen. Total DNA was isolated, phenol-chloroform-extracted,and dissolved in TE. Three micrograms DNA were blotted on positivelycharged Porablot plus membranes and measured as above. For controls,samples were treated with proteinase K, with RNase A (Life Technologies,Karlsruhe, Germany), or with DNase I (Invitrogen, NV Leek, Netherlands).Before blotting on membrane, DNase I treatment abolished the [³H]-signal, whereas RNase A and Proteinase K treatment were withouteffect.

Drug administration. Stock solutions were prepared in PBS/100% ethanol/bovine serum albumin (100:10:1) as vehicle. 5-Aza-'2-deoxycytidine(5-aza-dC) (Sigma, St. Louis, MO), an inhibitor of DNA methylation(Laird et al., 1995), was dissolved at a concentration of 10 µg/µl.Trichostatin A (TSA; Sigma), a specific inhibitor of histone deactylation(Yoshida et al., 1995), was dissolved at a concentration of 0.1and 1 µg/µl, respectively. Two microliters of the solution orvehicle were administered intracerebroventricularly (bregma $-$ 0.9mm lateral; $-$ 0.1 mm posterior; $-$ 3.1 mm deep) 10 min before ischemiausing a Hamilton syringe (Fisher Scientific, Pittsburgh, PA) asdescribed (Endres et al., 1998b). All inhibitor experiments wereperformed in 129/SV wild-typemice.

Determination of lesion size. Animals were killed at 72 hr reperfusion (30 min MCAo) or 24 hr reperfusion (2 hr MCAo), andbrains were snap-frozen in isopentane on dry ice for cryostatsectioning. Infarction areas were quantitated with an image analysissystem (M4, Imaging Research, St. Catherines, Ontario, Canada)on 20 µm hematoxylin and eosin (H&E)-stained cryostat sections.Infarction volume was calculated by summing the volumes of eachsection directly (Huang et al., 1994) or indirectly (only for2 hr MCAo experiments) using the following formula: contralateralhemisphere (mm³) $-$ undamaged ipsilateral hemisphere (mm³). The difference between direct and indirect infarct volumesreflects brainswelling.

Determination of neuronal survival. The density of viable cells with neuronal appearance was counted within ischemic striatumon coronal H&E-stained sections (20 µm) at the level of the anteriorcommissure using an established protocol (Fink et al., 1998).

Data analysis. Experiments (cerebral ischemia, evaluation of infarct size, cell counts) were performed in a blinded fashion.Data are presented as mean ± SE. Differences between groups wereevaluated by paired or unpaired two-tailed Student's t test orby ANOVA followed by Scheffe's test (physiology). p values of<0.05 were considered statisticallysignificant.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Effects of ischemia on MTase catalytic activity

We determined MTase catalytic activity ex vivo using an established model of 30 min MCAo followed by reperfusion (Endres etal., 1998b). As displayed in Figure 1A, cortical and striatallevels in ischemic tissue did not differ from baseline (sham)and contralateral tissues, nor did they change with time (1, 3,6, 18 hr) during reperfusion. Levels in Dnmt^S/+ mice were ~50% compared with Dnmt^+/+ mice and also did not change over time (1, 3, 6, 18 hr) (Fig.1B). Activity levels in cerebellum were considerably higher thanin other brain regions, which agrees with the literature (Brookset al., 1996). Hence, MTase, an enzyme with a short protein halflife (Szyf, 1994), remains functionally intact after ischemia/reperfusion.

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Figure 1. Time-dependent changes of MTase activity in Dnmt^+/+ (A) and Dnmt^S/+ mice (B) after 30 min middle cerebral artery occlusion and reperfusion. MTase activity was measured in ischemic cortex (COR) and striatum (STR) along with the respective contralateral tissue and sham (S)-operated animals. MTase activity was measured in nuclear extracts in vitro using a hemimethylated oligo-probe. Levels in cerebellum (CER) are shown for comparison. n = 2 animals per time point. Mean ± SE. p > 0.05.

Effects of ischemia on MTase protein levels

MTase protein was measured semiquantitatively using immunoblot analysis of brain lysates probed with rabbit antiserum (Tuckeret al., 1996a). A band corresponding to molecular weight 190 kDawas detected on immunoblot. MTase protein levels were ~50% inDnmt^S/+ mice compared with the wild-type strain in olfactory bulb (OB),striatum (STR), and hippocampus (HIP) (Fig. 2A). To characterizethe fate of MTase after brain ischemia, we measured MTase proteinafter 30 min MCAo/reperfusion. No differences were found overtime in ischemic striatum after recirculation of 0, 1, 3, 6, 12,18, 24, 48, and 72 hr (Fig. 2B). Hence, MTase levels did not changeover time after ischemia/reperfusion.

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Figure 2. A, MTase protein levels in olfactory bulb (OB), striatum (STR), and hippocampus (HIP) in brain lysates from normal (wt) and Dnmt^S/+ mice (s/+). Brain lysates were subjected to SDS-PAGE and immunoblot analysis performed using a polyclonal MTase antibody. The experiment was repeated three times; a representative experiment is shown. B, Time-dependent changes in MTase protein expression in striatum during reperfusion after 30 min middle cerebral artery occlusion. MTase protein was present in normal brain (sham) and did not change over time (0, 1, 3, 6, 12, 18, 24, 48, and 72 hr) between left (L = ischemic) and right (R = non-ischemic) hemispheres. The experiment was repeated three to four times per time point; a representative experiment for the time points 3, 6, and 18 hr is shown.

Effects of cerebral ischemia on DNA methylation in vivo

To measure newly incorporated methyl groups into DNA during brain ischemia/reperfusion in vivo, animals were first subjectedto 30 min MCAo, and on reperfusion a labeled methyl-group precursorof SAM (L-[methyl-³H]methionine) was administered. Twelve hours after reperfusion,DNA methylation was significantly higher in ischemic striatum(4.1-fold) and cortex (3.2-fold) compared with the respectivecontralateral tissues in wild-type mice (Dnmt^+/+ littermates) (Fig. 3A). DNA methylation, however, did not increasein ischemic tissue of Dnmt^S/+ mice (Fig. 3B). Together, these results demonstrate that methylgroup incorporation increases after ischemia/reperfusion in wild-typebut not in Dnmt^S/+ mice.

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Figure 3. Methyl group incorporation into brain DNA in vivo in Dnmt^+/+ (A) and Dnmt^S/+ mice (B) after 30 min middle cerebral artery occlusion. On reperfusion, L-[methyl-³H]methionine was administered and [³H]methyl group incorporation was measured after 12 hr. DNA methylation was significantly increased in ischemic cortex (COR) and striatum (STR) compared with the contralateral side in Dnmt^+/+ (A) but not Dnmt^S/+ mice (B). Levels in cerebellum (CER) are shown for comparison. n = 4 and 5 animals. Mean ± SE. *p < 0.05. Paired Student's t test.

Smaller cerebral lesions and improved neuronal survival in Dnmt^S/+ mice after mild stroke

To determine whether the failure to increase DNA methylation altered the susceptibility of Dnmt^S/+ mice to tissue injury, we quantitated lesion volume after 30min MCAo/72 hr reperfusion. In fact, lesion size was significantly(29%) reduced compared with controls (Fig. 4A). Moreover, whenneurons were counted within ischemic striatum, the density ofviable cells was 2.4-fold higher in the Dnmt^S/+ mice compared with controls (Fig. 4B). These results demonstratethat reduced MTase activity is beneficial during mild cerebralischemia.

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Figure 4. A, Infarct volume was 29% smaller in Dnmt^S/+ mice compared with Dnmt^+/+ mice after 30 min filamentous middle cerebral artery occlusion (MCAo) and 72 hr reperfusion. Brain lesion volume was determined on serial coronal hematoxylin and eosin-stained cryostat sections (20 µm). B, Dnmt^S/+ mice had significantly higher numbers of viable cells in ischemic striatum after 30 min MCAo/72 hr reperfusion compared with controls. Viable cells with neuronal appearance were counted on coronal sections (20 µm) through the anterior commissure. Mean ± SE. n = 14 and 15 animals per group. *p < 0.05 compared with Dnmt^+/+ mice. Student's t test.

Systemic physiological parameters are unaltered in Dnmt^S/+ mice

Because alterations in systemic and cerebrovascular parameters can modify outcome after stroke, we excluded possible effectsof such variables by careful physiological monitoring. Rectaltemperature, arterial blood pressure, pH, partial pressure ofoxygen and carbon dioxide before, during, and after ischemia didnot differ between groups (Table 1). rCBF, measured with a laserDoppler flow probe, decreased to <20% of baseline ischemia inall animals and returned to ~100% within 5 min after reperfusion(Table 1). Blood pressure after reperfusion was somewhat lowerin Dnmt^S/+ mice compared with controls (82 ± 6 vs 101 ± 5 mmHg) (Table 1).Differences in blood pressure after ischemia between groups couldpossibly be explained by specific gene expression changes (e.g.,of endothelial NO synthase); however, they are unlikely to explainimproved outcome in Dnmt^S/+ mice because systemic hypotension normally aggravates ischemicdamage (Harms et al., 2000).


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Table 1. Physiological variables at baseline and during ischemia in Dnmt^+/+ and Dnmt^S/+ mice

Pharmacological inhibition of DNA methylation and histone deacetylation confers stroke protection in wild-type mice

To test the theory that a pharmacological inhibitor of MTase confers stroke protection in wild-type mice, we treated 129/SVmice with the MTase inhibitor 5-aza-dC. Twenty micrograms givenintracerebroventricularly 10 min before 30 min MCAo reduced lesionvolume by 34% at 72 hr (Fig. 5). After a slightly different ischemiaprotocol (45 min MCAo followed by 48 hr reperfusion), lesion sizewas 54% smaller in the 5-aza-dC-treated animals (43.2 ± 12.6 vs19.9 ± 0.8 mm³ in control vs treated mice, respectively; p < 0.001; n = 4 pergroup). We also determined methyl group incorporation into DNA(12 hr reperfusion) in 5-aza-dC-treated aniimals versus vehicle-injectedanimals. For this experiment, 400 µl [methyl-³H]methionine without additional PBS was used. A 2.72-fold increasecompared with the contralateral side was found in the ischemicterritory of vehicle-injected animals (90 ± 14 vs 244 ± 75 dpmin contralateral vs ischemic tissue, respectively; 3 µg DNA; n= 4). However, in 5-aza-dC-treated animals this increase was only1.38-fold (101 ± 13 vs 140 ± 31 dpm in contralateral vs ischemictissue, respectively; 3 µg DNA; n = 3).

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Figure 5. Treatment with the MTase inhibitor 5-aza-2'-deoxycitide (5-aza-dC; 20 µg) or the specific deacetylation inhibitor trichostatin A (TSA; 1 or 10 µg) reduced lesion size after 30 min of filamentous middle cerebral artery occlusion and 72 hr of reperfusion compared with vehicle in 129/V mice. Drugs or vehicle was administered intracerebroventricularly 10 min before ischemia onset. Lesion volume was determined quantitatively. Data are presented as mean ± SE. n = 5-9 animals per group. *p < 0.01 versus vehicle. Student's t test.

Because deletion/inhibition of MTase may augment the level of gene transcription, we tested whether increasing gene transcriptionby a related yet distinct mechanism (i.e., inhibition of histonedeacetylation) (Yoshida et al., 1995; Eden et al., 1998; Joneset al., 1998; Nan et al., 1998) would also protect from ischemicbrain injury. Accordingly, when animals were pretreated with TSA,a highly specific inhibitor of histone deacetylase (Yoshida etal., 1995) (0.2 or 2 µg, i.c.v., given 10 min before ischemia),lesion size was significantly reduced after 30 min MCAo/72 hrreperfusion (Fig. 5). After 45 min MCAo/48 hr reperfusion, lesionsize was 48% smaller in TSA-treated animals (43.2 ± 12.6 vs 22.4± 1.2 mm³ in control vs 2 µg TSA, respectively; p < 0.001; n = 4 pergroup).

For both the 5-aza-dC and the TSA experiments, we observed no significant differences in physiological parameters betweengroups (rCBF, blood pressure, blood gases, rectal temperatures)that could influence ischemia outcome (n = 5 animals per group;ANOVA plus Scheffe's test; data notshown).

Damage after severe stroke is not blunted in Dnmt^S/+ mice

Excitotoxic and free radical-mediated mechanisms predominate after prolonged periods of ischemia presumably because of necroticmechanisms of cell death, whereas apoptotic mechanisms are unmaskedin milder forms of ischemia (Choi, 1988; Endres et al., 1997,1998b). We therefore tested the effects of dnmt1 heterozygosityin a model of severe stroke (2 hr MCAo andreperfusion).

First, we determined whether DNA methylation increases after more prolonged ischemia as it does after mild ischemia (30 minMCAo). Methyl group incorporation was not increased after 2 hrMCAo in wild-type mice (Fig. 6A). Moreover, there was no differencein infarct size between Dnmt^S/+ mice and wild-type littermates after 2 hr MCAo and 22 hr reperfusion(121.7 ± 11.5 vs 137.9 ± 19.6 mm³ in controls vs Dnmt^S/+, respectively; p > 0.05; n = 4 and 5). There was also no differencebetween groups when infarct size was corrected for brain swelling(Fig. 6B). Regional CBF during ischemia was <20% of baseline anddid not differ between groups (13.8 ± 3.1 vs 18.6 ± 3.0% in controlsvs Dnmt^S/+, respectively; p > 0.05; n = 4 and 5). Hence, DNA methylationdoes not increase after prolonged ischemia, and deletion of onegene copy of dnmt1 did not confer resistance to severe injuryas it did after brief periods of MCAo.

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Figure 6. A, Methyl group incorporation into brain DNA in vivo after 2 hr versus 30 min MCAo in 129/SV mice. On reperfusion L-[methyl-³H]methionine was administered, and [³H]methyl group incorporation into brain DNA was measured after 12 hr reperfusion. Unlike after 30 min MCAo (also see Fig. 3), DNA methylation did not increase in ischemic cortical tissue from the MCA territory compared with the contralateral side after 2 hr MCA occlusion. n = 5 (2 hr MCAo) and 4 (30 min MCAo) animals. Mean ± SE. *p < 0.05. Paired Student's t test. B, When Dnmt^+/+ and Dnmt^S/+ mice were subjected to 2 hr MCAo/24 hr reperfusion and infarct volume was quantitated, no difference in indirect infarct volume was noted between groups. This result was confirmed by a direct method to measure infarct volume (137 ± 19.6 vs 121.7 ± 11.5 mm³ for Dnmt^S/+ vs Dnmt^+/+ mice, respectively). Mean ± SE. n = 4 and 5. p > 0.05 compared with wild type. Student's t test.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

This is the first report to implicate DNA methylation in the evolution of ischemic brain injury. Ischemia/reperfusion generateda three- to fourfold increase in methyl group incorporation inbrain, whereas this increase was not observed in transgenic animalsexpressing reduced MTase levels; furthermore, the mutant brainwas resistant to injury as evidenced by decreased striatal damageand increased numbers of surviving striatal neurons. There wereno group differences in genetic background or differences in physiologicalor cerebrovascular parameters to explain these results. Together,this may mean that DNA methylation may render the tissue morevulnerable to ischemic injury and may increase as a consequenceof such injury. The former postulation is supported by the findingthat ischemic brain injury can be reduced by treatment with aninhibitor of DNA methylation, 5-aza-dC.

DNA methylation after cerebral ischemia

An in vivo methylation assay was developed to measure newly incorporated methyl groups into DNA using L-[methyl-³H]methionine as methyl donor. [³H]methyl groups became incorporated into DNA, and we expect thatmost of the incorporated methyl groups was added to cytosine residues,although thymine methylation is a theoretical possibility (Razinet al., 1970). Although there were significant differences inDNA methylation in vivo between Dnmt^+/+ and Dnmt ^S/+ mice after ischemia, baseline methylation (contralateral hemisphereand cerebellum) did not differ, which agrees with previous findingsin Dnmt^S/+ cells (Li et al., 1992, 1993; Laird and Jaenisch, 1996). Absolutenumbers for methylation frequency could not be obtained with ourassay [assuming that the endogenous SAM pool was completely replacedby [methyl-³H]-SAM and that [³H]methyl groups were incorporated only into CpG dinucleotides,we estimate the striatal methylation frequency as 4.5 × 10⁶ (control) vs 12.2 × 10⁶ (ischemia) per CpG dinucleotide]. Despite significant increasesin methyl group incorporation into DNA, protein amount and enzymaticactivity of MTase were unchanged after cerebral ischemia and reperfusion,although small differences may have been missed because of assaysensitivity. Possible explanations include induction of otherMTases, which seems unlikely, however, in view of the resultsin Dnmt ^S/+ mice. A more reasonable explanation is an increase in MTase substrate,i.e., hemimethylated DNA, the mechanisms of which are discussedbelow.

Ischemia-induced methylation may reflect MTase activity in neurons after DNA damage and repair. Ischemic stress facilitatesdeamination of 5'MeC leading to G-T mismatches. For example, afterforebrain ischemia, the mutation spectrum indicates that 58% ofmutants with base substitutions (or one-third of all mutations)involved G-T mismatches (Liu et al., 1996). MTase may remethylatecytosine residues after base-excision repair of mismatches (Brookset al., 1996; Brooks, 1998). Cui et al. (1999) reported specificDNA damage 15 min after focal ischemia (i.e., in the c-fos gene),most of which was effectively repaired 60 min after ischemia bybase-excision repair. Another important mechanism in this respectis the observation that the formation of oxygen radicals [i.e.,8-hydroxyguanine (oh8dG)] profoundly alters methylation of adjacentcytosines, suggesting a role for oxidative injury in the formationof aberrant DNA methylation patterns (Cerda and Weitzman, 1997).Interestingly, oh8dG levels increased fourfold after forebrainischemia (Liu et al., 1996), and we observed a 2.7- to 4.1-foldincrease of methylation in a focal model. However, it is unlikelythat this mechanism can solely explain methylation changes inour model. Moreover, the recent discovery of a DNA demethylase(Bhattacharya et al., 1999) and the notion that DNA methylationmay be a reversible biological phenomenon (Rachmandani et al.,1999) shed new light on DNA methylation in postmitotic cells suchas neurons. Notably, our preliminary results indicate that ischemicresistance was also enhanced in genetically engineered mice inwhich the dnmt1 gene was selectively deleted in neurons (M. Endres,G. Fan, and R. Jaenisch, unpublished observation). Alternatively,increased DNA methylation after brain ischemia could relate tomitotic activity and DNA replication in non-neuronal cells suchas glia or progenitor cells (Lee et al., 1996).

In addition, administration of 5-aza-dC, an inhibitor of MTase, was able to significantly inhibit DNA methylation when administeredintracerebroventricularly before ischemia. Notably, 5-aza-dC,which is known to easily penetrate cells (Chabor et al., 1983),requires incorporation into DNA to inhibit MTase (Laird et al.,1995). In accordance with the above discussed mechanisms for DNAmethylation in the adult ischemic brain, 5-aza-dC could be incorporatedinto DNA of replicating non-neuronal cells or newly repaired DNAof neurons (Brooks et al., 1996; Liu et al., 1996; Brooks, 1998;Cui et al., 1999).

Possible neuroprotective mechanisms

In our study we showed that suppression of DNA methylation conferred resistance to ischemia as well as specific inhibitionof histone deacetylation. An inhibitor of DNA methylation, 5-aza-dC,caused significant reduction in ischemic injury as did a deficiencyin dnmt1 gene expression. In addition to methylation, histonedeacetylation has also been linked to gene silencing and providesa second global mechanism by which genes are regulated (Yoshidaet al., 1995; Eden et al., 1998; Jones et al., 1998; Nan et al.,1998). In fact, the two mechanisms have themselves been linkedrecently by data showing that transcriptional repression by themethyl-CpG-binding protein MeCP2 involves a histone deacetylasecomplex (Eden et al., 1998; Jones et al., 1998; Nan et al., 1998).We infer from our data that DNA methylation and histone deacetylationalter gene expression after ischemia in such a way as to rendertissue susceptible to injury. According to a "good versus badgene" theory, this could relate to overexpression of protective/antiapoptoticgenes (e.g., c-fos, bcl-2, sod) or repression of deleterious/proapoptoticgenes (e.g., bad, bax). Cui et al. (1999) recently reported specificalterations in gene expression of c-fos after focal ischemia/reperfusion.Hence, neuroprotection may relate not only to the specific characteristicsof delayed neuronal cell death after mild stroke but to ischemia-inducedchanges in gene expression mediated by DNA methylation and histonedeacetylation. To further differentiate between possible necroticand apoptotic mechanisms, we used two different models of cerebralischemia (30 min vs 2 hr MCAo) (Endres et al., 1998b). The factthat methyl group incorporation did not increase after 2 hr MCAoand mutants partially deficient in MTase were not protected fromsevere stroke points to fundamental differences in the pathwaysof mild versus severe ischemicinjury.

Experiments using Dnmt^S/+ mice cannot distinguish between effects of dnmt1 heterozygosity during development versus effects inthe adult brain. However, the fact that methylation patterns aresimilar between Dnmt^S/+ and Dnmt^+/+ cells (Li et al., 1992, 1993; Laird and Jaenisch, 1996) and thatinhibiting MTase activity with 5-aza-dC was neuroprotective duringischemia suggests that effects in adult brain are responsiblefor protection. Experiments using conditional knockouts will helpto resolve thisissue.

In addition to the above epigenetic mechanisms, the enzyme MTase could enhance DNA mutagenesis. Under certain conditions,especially during SAM deficiency, C-T and C-U transitions canbe facilitated by MTase directly (Wyszynski et al., 1994; Gonzalgoand Jones, 1997). Possibly, the mutagenic potency of MTase iscompensated for by an effective DNA repair mechanism. This wouldimply a protective role for mismatch repair versus deleteriouseffects of MTase and DNA methylation. Therefore, although thismechanism has yet to be convincingly demonstrated in mammals,a direct genetic mechanism by which MTase contributes to ischemicdamage is possible. Notably, SAM administration is neuroprotectivein models of cerebral ischemia in rats and gerbils (Sato et al.,1988; Rao et al., 1997). It will be interesting to measure SAMlevels after cerebral ischemia and conditions of MTase deficiencyin ourmodel.

In conclusion, we demonstrate that DNA methylation increases in vivo after ischemia/reperfusion and that reduced levels ofMTase in brain protect from ischemic injury. These observationsunderscore the potential importance of DNA methylation to mechanismsof injury and repair in the postischemicbrain.

  FOOTNOTES

Received Nov. 11, 1999; revised Feb. 22, 2000; accepted Feb. 24, 2000.

This research was supported by Grant NS10828 from National Institutes of Health (M.A.M.), the Deutsche Forschungsgemeinschaft(En343/1-1 to M.E.; En343/4-1 to M.E. and A.M.; Me1562/1-1 toA.M. and U.D.; Di454/8-2 to U.D), the Humboldt-University of Berlin(M.E.), and the Hermann and Lilly Schilling Stiftung (U.D.). Wethank Guoping Fan for assistance in the immunoblotassays.
M.E. and A.M. contributed equally to thiswork.

Correspondence should be addressed to Dr. Matthias Endres, Department of Neurology, Charité Hospital, Humboldt-University,D-10098 Berlin, Germany. E-mail: matthias.endres{at}charite.de.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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