DNA Hypomethylation Perturbs the Function and Survival of CNS Neurons in Postnatal Animals

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The Journal of Neuroscience, February 1, 2001, 21(3):788-797

DNA Hypomethylation Perturbs the Function and Survival of CNS Neurons in Postnatal Animals
Guoping Fan¹, Caroline Beard¹, Richard Z. Chen¹, Györgyi Csankovszki¹^,², Yi Sun³, Marina Siniaia⁴, Detlev Biniszkiewicz¹, Brian Bates¹, Peggy P. Lee⁵, Ralf Kühn⁶, Andreas Trumpp⁷, Chi-Sang Poon⁴, Christopher B. Wilson⁵, and Rudolf Jaenisch¹^,²
¹ Whitehead Institute for Biomedical Research and ² Department of Biology, Massachusetts Institute of Technology, Cambridge, Massachusetts 02142, ³ Division of Neuroscience, Department of Neurology, Children's Hospital, Harvard Medical School, Boston, Massachusetts 02115, ⁴ Harvard-Massachusetts Institute of Technology Division of Health Sciences and Technology, Massachusetts Institute of Technology, Cambridge, Massachusetts 02139, ⁵ Departments of Immunology and Pediatrics, University of Washington, Seattle, Washington 98195, ⁶ Department of Genetics, University of Köln, Köln, Germany, and ⁷ G. W. Hooper Foundation, University of California, San Francisco, California 94143

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

DNA methyltransferase I (Dnmt1), the maintenance enzyme for DNA cytosine methylation, is expressed at high levels in the CNSduring embryogenesis and after birth. Because embryos deficientfor Dnmt1 die at gastrulation, the role of Dnmt1 in the developmentand function of the nervous system could not be studied by usingthis mutation. We therefore used the cre/loxP system to produceconditional mutants that lack Dnmt1 in neuroblasts of embryonicday 12 embryos or in postmitotic neurons of the postnatal animal.Conditional deletion of the Dnmt1 gene resulted in rapid depletionof Dnmt1 proteins, indicating that the enzyme in postmitotic neuronsturns over quickly. Dnmt1 deficiency in postmitotic neurons neitheraffected levels of global DNA methylation nor influenced cellsurvival during postnatal life. In contrast, Dnmt1 deficiencyin mitotic CNS precursor cells resulted in DNA hypomethylationin daughter cells. Whereas mutant embryos carrying 95% hypomethylatedcells in the brain died immediately after birth because of respiratorydistress, mosaic animals with 30% hypomethylated CNS cells wereviable into adulthood. However, these mutant cells were eliminatedquickly from the brain within 3 weeks of postnatal life. Thus,hypomethylated CNS neurons were impaired functionally and wereselected against at postnatalstages.

Key words: DNA methylation; Dnmt1; demethylation; neural development; cre/loxP system; respiration; epigenetic mechanism; gene regulation

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

DNA cytosine methylation in vertebrates influences many cellular events, including gene transcription, genomic imprinting,and genome stability (Jaenisch, 1997; Jones and Gonzalgo, 1997;Robertson and Wolffe, 2000). The DNA methylation pattern in adultcells is established during gametogenesis and early embryonicdevelopment via consecutive waves of demethylation and de novomethylation (Monk et al., 1987). A family of DNA (cytosine-5)methyltransferases (Dnmts) has been identified that catalyzesthe reaction of cytosine methylation in DNA (Bestor et al., 1988;Okano et al., 1998; Lyko et al., 1999; Okano et al., 1999). Thefirst cloned family member, Dnmt1, encodes a maintenance DNA methyltransferase(Dnmt1; EC 2.1.1.37) that preferentially methylates hemi-methylatedDNA that is generated after DNA replication (Bestor et al., 1988).The essential role of Dnmt1 in maintaining DNA methylation hasbeen demonstrated by targeted mutation of the Dnmt1 gene, whichresults in demethylation of the DNA in Dnmt1-deficient cells (Liet al., 1992; Lei et al., 1996). Dnmt1 mutant embryos die betweenembryonic day 8 (E8) and E10.5, indicating that DNA methylationis essential for embryogenesis (Li et al., 1992; Lei et al., 1996).The cause of lethality is not clear, but Dnmt1-deficient embryosexhibit numerous apoptotic cells in many tissues, including brainand liver, suggesting that DNA hypomethylation ultimately mayinduce an apoptotic pathway (Li et al., 1992). DNA methylationhas been shown to play an essential role in the transcriptionalregulation of imprinted genes (Li et al., 1993), the X-chromosome-linkedXist gene (Beard et al., 1995; Panning and Jaenisch, 1996), andretroviral intra-cisternal A particles (IAP) (Walsh et al., 1998).

The role of DNA methylation in neural development and function has not been explored. Interestingly, the mammalian brain expresseshigh levels of Dnmt1 both during development and in adulthood(Goto et al., 1994; Brooks et al., 1996; Trasler et al., 1996;Inano et al., 2000). The level of DNA methylation is higher inadult brain than in other tissues (Wilson et al., 1987; Tawa etal., 1990; Ono et al., 1993). Perinatally, DNA methylation levelsin the brain undergo a dynamic change (Tawa et al., 1990), suggestinga role for DNA methylation in the differentiation process of thebrain. Further evidence comes from a study of neuronal differentiationin PC12 cells that showed that treatment with a demethylatingagent 5-azacytidine blocks neurite outgrowth and upregulates theexpression of Id family transcription factors (Persengiev andKilpatrick, 1996, 1997). Recently, DNA methylation has been associatedwith at least three mental retardation diseases, including theRett, ICF, and the fragile X syndromes (for review, see Robertsonand Wolffe, 2000). The neurodevelopmental disease Rett syndromeis caused by mutations in the MECP2 gene, a methylcytosine-bindingprotein (Amir et al., 1999). Because a major function of the MECP2protein is to mediate methylation-induced gene suppression (Ngand Bird, 1999), the adverse effect of MECP2 mutations on braindevelopment suggests that changes in DNA methylation also mayaffect the postnatal CNS development. Endres et al. (2000) showedthat DNA methylation activity increases with transient ischemiaand contributes to brain injury, suggesting that levels of DNAmethylation influence adult CNS neuron survival under stressconditions.

Dnmt1-deficient embryos die around midgestation before neuronal differentiation (Li et al., 1992; Lei et al., 1996), precludingthe study of DNA methylation in brain development. We thereforeused the cre/loxP binary system to produce conditional knock-outmice in which the Dnmt1 gene deletion can be achieved in eitherbrain precursor cells at E9-E12 or in postnatal CNS neurons thathave exited the cell cycle. We demonstrated that, although Dnmt1is dispensable for postmitotic neurons, Dnmt1 deficiency in brainprecursor cells resulted in significant DNA hypomethylation inprogeny cells, including descendant postmitotic neurons. Mutantmice carrying 95% of hypomethylated cells in the CNS died becauseof respiratory distress, suggesting that DNA hypomethylation perturbsvital CNS functions that are required for postnatal life. Mutantmice with 30% of hypomethylated cells survived into adulthood;however, these hypomethylated cells were eliminated rapidly fromthe CNS during early postnataldevelopment.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Brain-specific Dnmt1 conditional mutant mice. We used the cre/loxP binary system to generate Dnmt1 conditional mutants. Detailsof generating the Dnmt1 conditional allele (Dnmt1^2lox) are reported elsewhere (Jackson-Grusby et al., 2000). Briefly,in this line of mice exons 4 and 5 of the Dnmt1 gene were flankedby loxP sites. Cre-mediated deletion of exons 4 and 5 would leadto out-of-frame splicing from exon 3 to exon 6, resulting in anull Dnmt1 allele (Jackson-Grusby et al., 2000). To achieve Dnmt1gene deletion in CNS precursor cells in vivo, we crossed the animalscarrying the Dnmt1^2lox conditional allele with the nestin-cre transgenic mice. The productionof nestin-cre transgenic mice has been described previously (Bateset al., 1999; Trumpp et al., 1999). For conditional gene deletionin postmitotic CNS neurons, we used the CamK-cre transgenic micein which the cre expression is under the control of the neuronalcalmodulin-kinase II $alpha$ (CamK) promoter. We also characterized thedistribution of cre-mediated gene deletion by crossing the CamK-creand nestin-cre transgenic mice with the lacZ reporter strainsas described by Akagi et al. (1997) and Soriano (1999). Briefly,the brain sections from different stages of transgenic mice wereprocessed for X-gal staining as described (Trumpp et al., 1999).The positive blue cells indicate places at which the cre-mediatedloxP recombination occurred (see Fig. 3 in Results) (Akagi etal., 1997; Soriano, 1999).

Some of the conditional mutants also carried the previously described Dnmt1 mutant N- and C-alleles (Dnmt1^N or ^C), which represent Dnmt1 hypomorphic (~2% Dnmt1 proteins) andnull alleles, respectively (Li et al., 1992; Lei et al., 1996).Southern blot analysis and PCR reactions were used for genotypingmice.

Southern and Northern blot analysis. DNA samples were extracted from brain tissues as previously described (Laird et al.,1991). RNA samples were purified with an RNAzol reagent (Tel-Test,Friendswood, TX) according to the manufacturer's procedure. DNAor RNA samples were subjected to electrophoresis and transferredto a nylon membrane (Zetabond). Hybridization of the blot wasperformed by the Quickhyb protocol (Stratagene, La Jolla, CA).Details of various DNA probes have been reported (Tucker et al.,1996; Jackson-Grusby et al., 2000). PhosphorImager (Fuji, Tokyo,Japan) and densitometry (Bio-Rad, Hercules, CA) analysis of theintensity of Dnmt1^2lox and Dnmt1^1lox alleles was used to quantify the efficiency of Dnmt1 gene deletionby the CamK-cre and nestin-cretransgenes.

Western blot analysis. Brain tissue lysates were separated by 7.5% SDS-PAGE gels, using a Bio-Rad minigel apparatus. One gelwas stained with Coomassie blue to visualize whether the proteinloading in each lane was even. A duplicate gel was blotted toa nylon membrane by electrotransfer for Western blotting. Theprocedure of Western blotting has been described (Fan and Katz,1993). Briefly, the membrane blot was blocked in 5% milk in Tris-bufferedsaline and incubated with Dnmt1 primary antibodies [Dnmt1 ATG4Ab, the rabbit anti-N-terminal Dnmt1 peptide; Dnmt1 C-term Ab,chicken anti-Dnmt1 catalytic domain peptide; see Gaudet et al.(1998) for detailed information on the antibodies], followed byperoxidase-conjugated secondary antibodies, and was visualizedwith enhanced ECL reagents (Amersham, Arlington Heights,IL).

Histological examination and TUNEL staining. Tissues dissected from mutant and control mice were fixed in 4% paraformaldehyde/PBSovernight and embedded in OCT for frozen sections or processedwith a VIP tissue processor (Miles, Elkhart, IN) for paraffinsectioning. Serial sections were stained with hematoxylin/eosinor cresyl violet for light microscopy. For cell death analysisthe TUNEL staining was performed either with a commercial in situcell death detection kit (Boehringer Mannheim, Indianapolis, IN)or by the terminal labeling of biotinylated dNTPs with the TdTenzymes (Life Technologies, Gaithersburg, MD) as described (Ben-Sassonet al., 1995), followed with avidin-peroxidase reactions as describedin the ABC kit (Vector Laboratories, Burlingame,CA).

Cortical and cerebellar cell cultures. Cortices from fetal brains (E15-E18) were dissected, treated with trypsin or papain,dissociated, and plated on coated glass coverslips, as previouslydescribed (Bonni et al., 1997). Detailed protocol of cerebellarcultures has been reported (Datta et al., 1997). At the time ofplating, recombinant adenoviruses carrying the cre transgene wereadded into cultures at a multiplicity of infection (MOI) ratioof 10:1 (virus/cell). Cultures were harvested at different timepoints for Western and Southern blotanalyses.

Immunocytochemistry and whole-mount immunohistochemistry. Cultured cells were fixed with 4% paraformaldehyde and permeabilizedwith Triton X-100. Monoclonal $beta$ -tubulin antibody (TuJ1) and polyclonalnestin antibodies [kindly provided by Drs. A. Frankfurter (Charlottesville,VA) and R. McKay (Bethesda, MD)] were applied and visualized withfluorescein-conjugated secondary antibodies. For whole-mount stainingof the diaphragm the tissues were fixed with 2% paraformaldehydeovernight, blocked in 5% goat serum with 1% DMSO overnight, andthen consecutively incubated with anti-neurofilament 150 (Chemicon,Temecula, CA) and FITC-conjugated secondary antibodies. Rhodamine-conjugated $alpha$ -bungarotoxin (Molecular Probes, Eugene, OR) was used to labelpostsynaptic AChR in the muscle. The preparations were observedon a Zeiss fluorescencescope.

Xist fluorescence in situ hybridization analysis. Cells were grown on glass coverslips, fixed in 4% paraformaldehyde, andstored in PBS. Hybridization, washing, and detection of probeshave been described (Panning and Jaenisch, 1996). Briefly, coverslipswere extracted with cytoskeletal buffer containing 0.5% TritonX-100, dehydrated, and incubated with the nick translation probeat 37°C overnight. Slides were washed at 39°C for three timesin 2× SSC/50% formamide, three times in 2× SSC, and twice in 1×SSC for 5 min each. Biotinylated probes were detected in 2 mg/mlBSA/4× SSC at 37°C for 30 min, using FITC-avidin. Fluorescentimages were captured either by a Nikon scope with Scanlytic systemor on Kodak Ektachrome 1600 slide film with a ZeissAxioskop.

Electrophysiology. Newborn mice were anesthetized with a light dose of sodium pentobarbital (Nembutal; 25-30 mg/kg, i.p.)(Paton et al., 1994) and were placed supine on a heating pad withthe temperature regulated at ~38° C (CWE C-831 Temperature Controller).Central respiratory activity was monitored by recording hypoglossalnerve discharge. A hypoglossal (XII) nerve (which innervates boththe genioglossus muscle and tongue retractors) was isolated byblunt dissection with a ventral approach at the cervical level,cut distally, mounted on custom-made bipolar silver-wire electrodes,and kept in a warm mineral oil pool. Inspiratory-related efferentneuronal discharges of the hypoglossal nerve were amplified (CyberAmp380, Axon Instruments, Foster City, CA), time-averaged with aleaky integrator (Paynter filter; time constant, 15 msec), andrecorded (Thermal Array Recorder, Nihon Kohden, Tokyo, Japan).In some experiments small custom-made bipolar fish-hook electrodeswere implanted into the diaphragm to record an electromyogram(EMG). Immediately after birth, small stainless steel electrodeswere implanted subdermally on both sides of the chest to recordan electrocardiograph (EKG). In some experiments the EKG was recordedin normal and mutant pups in utero with the mother under urethaneanesthesia (1.2 gm/kg, i.p.).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In vitro survival of postmitotic neurons in the absence of Dnmt1

Previous studies have shown that Dnmt1 transcripts and proteins were highly expressed in the CNS during embryogenesis andin adulthood. A recent study further demonstrated that the enzymeis localized primarily in the cytoplasm of neurons (Inano et al.,2000). To determine the role of Dnmt1 in postmitotic neurons,we used the cre/loxP system to delete the Dnmt1 gene conditionally(Fig. 1A). A conditional allele (referred to as Dnmt1^2lox), in which exons 4 and 5 of the Dnmt1 gene are flanked by loxPsites, was generated via gene targeting in embryonic stem (ES)cells. Expression of cre-recombinase causes the deletion of exons4 and 5, which results in a null allele of Dnmt1 (designated asa Dnmt^1lox allele; Jackson-Grusby et al., 2000).

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Figure 1. Conditional deletion of the Dnmt1 gene in postmitotic cerebellar neurons. A, Schematic drawing of the cre/loxP-mediated Dnmt1 gene deletion. In the Dnmt1^2lox allele exons 4 and 5 were flanked by the 34 bp loxP sequence. In the presence of cre-recombinase the two loxP sites recombined, resulting in deletion of the exons and creation of the Dnmt1^1lox null allele. B, P6 Dnmt1^2lox/2lox cerebellar dissociates were infected with recombinant adenovirus carrying the cre transgene at the time of plating and then were cultured for 1 d (1d) to 14 d (14d). DNAs were extracted from the cultures and digested with SpeI for Southern blot analysis of the efficiency of the Dnmt1 gene deletion in cerebellar cultures over time. The ratio of recombined null allele (1lox) over the sum of functional Dnmt1^2lox (2lox) and 1lox alleles indicates the efficiency of gene deletion. C, Western blot analysis of Dnmt1 proteins in control and mutant neurons. Top, Levels of Dnmt1 protein were detected with Dnmt1 antibodies in cultured cerebellar neurons with or without adeno-cre infection. Bottom, A duplicate gel was stained with Coomassie blue staining to show the equal loading of the protein extracts. D, Southern blot analysis of DNA methylation in cerebellar cultures. DNAs were digested with the methyl-sensitive enzyme HpaII, separated on agarose gel, transferred to the membrane, and hybridized with a centromeric minor satellite repeat probe. Small-molecular-weight fragments in Dnmt1 mutant embryonic stem cells indicate extensive demethylation of their DNA.

We first examined whether the Dnmt1 protein turns over in postmitotic cerebellar neurons. Dnmt1 protein was detected readilyin dissociated cerebellar granule neurons from control Dnmt1^2lox/2lox animals by Western blot analysis (Fig. 1C). In fact, levels ofDnmt1 in these cells were comparable with those in dividing embryonicfibroblasts (data not shown; see also Inano et al., 2000). Whencerebellar cultures containing Dnmt1^2lox/2lox cells were infected with adenoviruses carrying the cre transgene(adeno-cre), deletion of the Dnmt1 gene occurred in 60% of culturedcells within 24 hr (Fig. 1B). Gene deletion was completed at 100%efficiency within 3 d of adenovirus infection (Fig. 1B). In parallelto the time course of gene deletion, Dnmt1 protein levels weredecreased significantly within 24 hr and virtually undetectableby the end of 3 d in culture (Fig. 1C). No Dnmt1 proteins weredetected by Western blot analysis in adeno-cre-infected neuronsafter 5-7 d, using antibodies against either the N terminus (Fig.1C) or C terminus of Dnmt1 (data not shown). This result indicatesthat the enzyme undergoes a rapid turnover in postmitotic cerebellarneurons.

To determine the consequence of Dnmt1 deficiency on levels of DNA methylation and neuronal survival, we examined culturedcerebellar neurons with the Dnmt1 gene deletion for a period of2 weeks. These neurons apparently survived well in the absenceof Dnmt1 during the 2 weeks of the culture period. Immunostainingwith neuron-specific $beta$ -tubulin antibody (TuJ1) indicated thatthe neurons were healthy, with extensive neurite outgrowth (Fig.2). Southern blot analysis indicated that the depletion of Dnmt1did not change global DNA methylation (see Fig. 1D).

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Figure 2. Survival of cerebellar neurons in the absence of Dnmt1. P6 Dnmt1^2lox/2lox cerebellar dissociates were infected with adeno-cre at the beginning and were cultured for 2 weeks. These neuron-enriched cultures were double-stained with neuron-specific $beta$ -tubulin III (TuJ1) antibodies (red) to visualize extensive neurites and with DAPI (blue) to show the healthy neuronal nuclei. Scale bar, 45 µm.

Conditional deletion of Dnmt1 in postmitotic CNS neurons in vivo

Although the above results showed that Dnmt1 is not essential for maintaining global DNA methylation and neuronal survivalin vitro, it is unclear whether Dnmt1 is required for the survivalof postmitotic neurons in vivo. We therefore crossed the Dnmt1^2lox allele with a strain of CamK-cre (line 93) transgenic mice thatexpress cre in postmitotic neurons from the perinatal stage. CamK-cre-mediatedgene deletion in CNS neurons was confirmed first by a lacZ reportergene (Akagi et al., 1997). Gene deletion was detected in a smallnumber of forebrain neurons perinatally and reached the peak levelafter 3 weeks postnatally (data not shown). As shown in Figure3A-D, in 3-week-old transgenic mice CamK-cre-mediated gene deletionwas widespread in the forebrain, including the cortex, hippocampus,and striatum, but virtually absent in the cerebellum (except ina few scattered Purkinje cells). The blue cells were morphologicallyCNS neurons, confirming the neuronal specificity of the CamK-cretransgene. The spatial and temporal distribution pattern of thelacZ-positive cells in the CamK-cre;lacZ reporter transgenic micewas well confirmed by Southern blot analysis of the efficiencyof Dnmt1 gene deletion in various brain regions of CamK-cre;Dnmt1conditional mutants, suggesting that CamK-cre-mediated Dnmt1 genedeletion occurs in a similar pattern as observed with the lacZreporter gene. Conditional Dnmt1 mutants were recovered at theexpected Mendelian ratio, indicating that Dnmt1 deficiency inpostmitotic CNS neurons did not affect animal viability. Southernblot analysis showed that Dnmt1-deficient neurons were presentin adult mutant brains at all of the stages that were examined,ranging from 3 to12 weeks, 8 months (Fig. 3E), and up to 17 monthsof age, which is the last time point that was analyzed (data notshown). The efficiency of gene deletion in the cortex of conditionalmutant mice was similar to that in control conditional heterozygousmice (both at ~50%; see Fig. 3E). In addition, the percentageof Dnmt1-deficient neurons in most brain regions, except the olfactorybulb, was constant during postnatal life (Fig. 3E), suggestingthat Dnmt1 deficiency in postmitotic neurons was not detrimentalto long-term neuronal survival.

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Figure 3. Survival of cortical neurons in the absence of Dnmt1 in vivo. A-D, X-gal staining of brain sections from a 3-week-old mouse carrying the CamK-cre transgene and a lacZ reporter gene under the control of the $beta$ -actin promoter (Akagi et al., 1997). The cells positive for $beta$ -gal enzymes (blue cells) represent those neurons having undergone cre-mediated gene recombination events. Scale bar, 675 µm. E, Southern blot analysis of cortex DNAs from conditional CamK-cre;Dnmt^2lox/+ (2lox/+) heterozygous and CamK-cre;Dnmt1^2lox/C mutant animals (2lox/C). Note that the wild-type (WT) and null C-alleles were detected at the same size in this blot. The genotypes of wild-type and C-alleles were ascertained by the absence and presence of the neomycin gene in the Dnmt1 locus. F, Methylation analysis in cortex DNAs. IAP, Intra-cisternal A particle retrovirus; MMLV, Moloney murine leukemia virus.

The long-term presence of Dnmt1-deficient neurons in CamK-cre;Dnmt1 conditional mutants allowed us to examine whether globalDNA methylation would change in vivo over a time course of months.Southern blot analysis of DNA methylation of endogenous retroviralrepeats [IAP and Moloney murine leukemia virus (MMLV)] did notshow any obvious demethylation in mutant neurons that had lackedDnmt1 for 8 months (Fig. 3F). These data indicated that Dnmt1is not essential for maintaining global DNA methylation in postmitoticneurons in vivo.

Dnmt1 deficiency in CNS precursor cells in vivo causes global DNA hypomethylation and neonatal death of mutant animals

We next examined the consequence of the Dnmt1 gene deletion in CNS precursor cells in vivo. For this, we crossed Dnmt1^2lox females with male mice carrying a nestin promoter-driven cretransgene that is activated in CNS precursor cells at E9-E10 andresults in almost complete gene deletion by midgestation (Bateset al., 1999; Trumpp et al., 1999).

Mutant mice were obtained at the expected Mendelian frequency at all of the embryonic stages that were examined (E10.5-E19.5)but were never recovered postnatally. Careful observation of mutantmice delivered either naturally or by Cesarean section at E18.5-E19.5revealed that neonatal mutant mice died within 1 hr of birth becauseof respiratory failure (see below). Southern blot analysis ofE19.5 mutant embryos showed that the cre-mediated gene deletionof Dnmt1 had occurred in ~95% of the cells in the CNS (Fig. 4A),in agreement with previous observations (Bates et al., 1999).Moderate gene deletion (<30%) was observed in muscles and kidney,and a low frequency of gene deletion was seen in lung, heart,and liver (Fig. 4B). Cre-mediated Dnmt1 deletion was already detectableat E10.5 (data not shown) and was complete at E12.5 in the brain(Fig. 4B). Importantly, the proportion of brain cells carryingthe Dnmt1 gene deletion remained constant throughout later stagesof embryonic development (Fig. 4B), suggesting that Dnmt1-deficientcells survived throughout embryogenesis. Western blot analysisshowed that levels of Dnmt1 proteins were decreased greatly atE12.5 and were undetectable at E15.5 (Fig. 4C), suggesting thatthe enzyme turned over rapidly after gene deletion. It is worthnoting that neurogenesis is the major event in the brain duringembryonic development, and gliogenesis in the CNS mainly occurspostnatally (Cepko et al., 1990; Mission et al., 1991; Cavinesset al., 1995). Thus, the majority of Dnmt1-deficient brain cellsin conditional mutant embryos is expected to be postmitotic CNSneurons.

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Figure 4. Deletion of the Dnmt1 gene in the brain by the paternally inherited nestin-cre transgene. A, Southern blot analysis of the efficiency of the nestin-cre-mediated Dnmt1 gene deletion in various brain regions and peripheral tissues from E19.5 conditional knock-outs. PhosphorImager analysis of mutant Dnmt1^1lox (1lox) alleles and functional Dnmt1^2lox (2lox) alleles indicated a recombination efficiency of ~95% in the brain. Approximately 10-30% recombination was detected in intestine, limb, cranial muscles, and kidney. Only very minor amounts (<5%) of recombination were detected in lung, heart, and liver. B, Dnmt1 gene deletion in E12.5-E18.5 brain tissues. DNA samples were collected from embryos carrying a paternally derived nestin-cre transgene and Dnmt1 alleles as indicated (heterozygous control, 2lox/+; mutant, 2lox/2lox or 2lox/N). PhosphorImager analysis showed that ~95% of the Dnmt1^2lox allele was recombined into the null Dnmt1^1lox allele in the brain from E12.5 to E18.5. C, Western blot analysis of Dnmt1 proteins in control and mutant brain tissues. Brain extracts from E12.5, E15.5, and E18.5 embryos were probed with a specific antibody against the N terminus of the Dnmt1 protein. A duplicate gel was stained with Coomassie blue as a loading control. Note that the E18.5 control sample was from a Dnmt1^2lox/N embryo, which showed a reduced level of Dnmt1 proteins as compared with Dnmt1^2lox/2lox control samples at E12.5 and E15.5. con, Control samples; mut, mutant samples.

To assess the effect of Dnmt1 deficiency on genomic methylation, we digested brain DNA with the methylation-sensitive enzymeHpaII and probed the Southern blots with a centromeric minor satelliterepeat probe (Fig. 5A) or an IAP DNA fragment (Fig. 5B). Theseprobes detect multiple copies of repeated DNA sequences that arehighly methylated in wild-type mice. As indicated by the low-molecular-weightfragments in Figure 5, A and B, there was substantial demethylationin the brain of mutant embryos at E12.5 or older because of thedeletion of the Dnmt1 gene. We also detected methylation changesin single-copy genes. As shown in Figure 5C, significant demethylationwas observed at several methylation sites surrounding the codingexon of the bdnf gene. From the densitometry analysis the proportionof demethylated DNA fragments was estimated to be ~30-40%. Althoughsubstantial DNA hypomethylation occurred in mutant brains fromE12 on, CNS development seemed to proceed normally. A histologicalsurvey of mutant embryos at different embryonic stages did notshow any obvious defect in the brain structure. Mutant brainsat E15.5 also did not show any obvious increase in cell deathas assessed by TUNEL staining (data not shown).

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Figure 5. Dnmt1 deficiency results in global genomic hypomethylation. A, B, Southern blot analysis of DNA methylation in the brain. The same DNA samples in Figure 1C were used for the methylation assay. DNA was digested with methyl-sensitive enzyme HpaII or methyl-insensitive enzyme MspI (-CCGG-) and was hybridized with a centromeric minor repeat probe (A) or an IAP probe (B). The appearance of small-molecular-weight DNA fragments indicates demethylation at the CpG sites of centromeric repeats or IAP retroviruses in the genome. con, Nestin-cre;Dnmt1^+/2lox; mut, Nestin-cre;Dnmt1^{2lox/2lox or
2lox/N}; $-$ / $-$ ES cells, Demethylated DNA samples from Dnmt1 null embryonic stem cells (Lei et al., 1996). C, Brain DNA from E18.5 embryos was digested with SacI and HpaII enzymes and the probe with a 750 bp BDNF cDNA.

To assess the effect of DNA hypomethylation in vitro, we examined the survival and differentiation of mutant cortical neuronsin dissociated cell culture at E15.5. Mutant and control corticalcells were cultured for 24 or 96 hr. After 1 d in culture ~80%of the cells were postmitotic neurons expressing neuronal-specific $beta$ -tubulin, and the remaining 20% of the cells were precursor cellsexpressing the nestin intermediate filament marker that predominantlydifferentiated into glial-like cells in our culture conditions(Fig. 6A,B). After 4 d in culture the composition of both thewild-type and mutant cultures had changed to ~50% neurons and50% glial-like cells because of active proliferation and differentiationof precursor cells and decreased survival of neuronal cells (Fig.6C,D). Analysis of global DNA methylation confirmed that culturedcells remained hypomethylated throughout the culture period (Fig.6E). No difference was found in neuronal survival between themutant and control cortical cells after either 24 or 96 hr inculture, indicating that Dnmt1 deficiency and DNA hypomethylationdid not affect neuronal survival in vitro at this embryonic stage(Fig. 6A-D). Our results are consistent with the notion that genomichypomethylation has no detectable effect on the survival of embryoniccortical neurons.

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Figure 6. Survival of hypomethylated cortical neurons in vitro. A-D, E15.5 cortical cells from control animals (con, Dnmt^2lox/2lox in A and C) and Nestin-cre;Dnmt1^2lox/2lox mutants (mut, in B and D) after 24 or 96 hr in culture. Cultured cells were double-stained with a monoclonal TuJ1 antibody against neuronal-specific $beta$ -tubulin III (green) and a polyclonal antibody against nestin intermediate filaments for precursor cells (red). Note that in 24 hr cultures ~80% of cells were postmitotic neurons. In 96 hr cultures the neurons and glial-like cells (nestin-positive) were ~50% each, and no difference in these ratios was observed between control and mutant cultures. Scale bar, 60 µm. E, DNA hypomethylation in cultured E15.5 cortical cells. DNAs from cortical cells cultured for 24 or 96 hr were assayed for global demethylation by probing with IAP retro-elements. Demethylated IAP DNA fragments were detected readily in the mutant cultures. con, Control Dnmt^2lox/2lox cultures; mut, conditional knock-out cultures.

We also examined DNA hypomethylation at individual cell levels by using dissociated cortical cultures. It has been shown thatthe Xist gene on the active X chromosome is silenced by methylationat the time of X inactivation but is activated by demethylation,leading to ectopic X inactivation (Beard et al., 1995; Panningand Jaenisch, 1996). In female cells Xist mRNA is expressed fromand associated with the inactive X in every cell. Fluorescencein situ hybridization (FISH) analysis showed that a strong XistmRNA signal was detected in all of the neurons explanted fromthe brain of E15.5 control females, but not from control maleembryos (Fig. 7). In contrast, a strong Xist mRNA signal, similarto the one seen in the control female cells, was seen in a portionof neurons explanted from mutant male embryos (Fig. 7, third panel).Quantification of Xist-expressing cells showed that ectopic Xistactivation occurred in 4-8% of mutant cells explanted at E15.5and E19.5 that had been cultured for 1-7 d (Table 1).

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Figure 7. Expression of Xist mRNA in neuronal and glial cells in culture. Xist FISH analysis was performed as described in Materials and Methods. Xist RNA expression (red dots in DAPI-stained blue nuclei) was detected in a portion (4-8%) of male mutant cells in 1-d-old E15.5 cortical neuronal cultures (also see Table 1). A few mutant cells also express the Xist transcripts in distributed granules within the cells (third panel), characteristic of cells in the early G₁ phase of cell cycle (Clemson et al., 1996). con, Control embryos (Dnmt1^2lox/2lox); mut, conditional mutant embryos. Scale bar, 7 µm.


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Table 1. Number of Xist-expressing cells in male mutant cortical cultures

Dnmt1 deficiency and DNA hypomethylation result in defects in neuronal respiratory control

To assess the possible cause of lethality in neonatal mutant mice that lack Dnmt1 in the brain, we examined E18.5 and E19.5mutant mice delivered by Cesarean section. In contrast to thecontrol mice that survived after the Cesarean section, all mutantmice died within 1 hr of delivery. Although mutant mice occasionallygasped, they did not initiate coordinated rhythmic breathing.Postmortem examination showed that their lungs failed to inflate,confirming respiratory failure (data notshown).

Multiple causes could lead to respiratory failure, including a defect in neural rhythmogenesis or motor output of the respiratorypattern generator, occlusion of the respiratory tract, delay inlung development, or abnormalities secondary to the failure ofthe cardiovascular or other vital systems. We first examined thebehavior of mutant fetuses within the uterus. Mutant mice in uterohad normal body movement, either spontaneous or in response tomechanical stimuli such as a pinch, suggesting that they had anormal sensorimotor reflex. We also monitored EKGs of the heartin utero and found a normal heart rate in mutant mice (control,356/min; mutant, 346-364/min). This suggests that respiratoryfailure in mutant animals was not caused by malfunction of thecardiovascular system. At the light microscope level the morphologyof various lung cells in conditional mutant animals appeared normal(data not shown). This is consistent with the observation thatlittle of Dnmt1 gene deletion was observed in the lung (see Fig.4A). Similarly, histological examination did not show any obviousabnormalities in respiratory muscle groups, including the intercostaland diaphragm muscles. In addition, diaphragm muscles were innervatednormally by the respiratory phrenic nerve originating from thecervical spinal cord (data not shown). These observations suggestthat the respiratory failure in the mutant was not caused by abnormalitiesof the peripheral respiratorysystem.

To investigate whether the respiratory failure in the Dnmt1 mutants was caused by a defect in the neural control of respirationin the CNS, we monitored the neuronal activity of the 12th cranialhypoglossal nerve and performed a diaphragmatic electromyogramin E18.5 and E19.5 mice delivered by Cesarean section. It is knownthat the majority of hypoglossal neuronal discharges is inspiratory,with a bursting period similar to that of phrenic nerve activity.Indeed, many hypoglossal motor neurons receive innervations frompremotor inspiratory neurons located within the respiratory patterngenerator in the ventrolateral medulla (Withington-Wray et al.,1988; Ono et al., 1994) (for review, see St. John, 1998). Figure8A shows that the hypoglossal nerve activity in normal mice displayeda rhythmic but gasping-like pattern ~5 min after birth (frequency,12/min), which was converted to an eupneic pattern with increasedrespiratory frequency (50/min) and heart rate (260/min) within10-20 min. In contrast, mutant mice at birth produced only sporadicgasping activity, which never developed into an eupneic pattern(Fig. 8A). Although occasionally showing arrhythmia, the initialheartbeat rate in mutant mice was close to that of control animalsimmediately after birth. Some 20-30 min after delivery, however,the heartbeat of mutant mice became increasingly irregular andsporadic (~30/min), and the animals died shortly thereafter.

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Figure 8. Lack of respiratory drive in the 12th cranial nerve. A, Electrophysiological recordings of descending respiratory discharge from hypoglossal nerve. Control (con, Dnmt1^2lox/2lox) and conditional mutant mice were dissected from the uterus at E18.5 and E19.5 and immediately prepared for 12th nerve recording as described in the Materials and Methods. Only occasional spontaneous gasping was observed in mutant mice. The gasping discharge also could be induced occasionally by tail pinching of mutant mice when an initial recording did not show any spontaneous signals. Similar results were obtained with six control and five mutant mice. Insets for each trace are EKG recordings obtained with subcutaneous electrodes (the EKG in the second control trace was derived from the diaphragmatic EMG recording). B, Normal morphology of hypoglossal motor neurons in the brainstem. E18.5 control (CON) and mutant embryos were fixed with 10% formalin and processed for paraffin histology. Brain sections were stained with cresyl violet. No obvious morphological difference was observed between control and mutant hypoglossal motor nuclei. Scale bar, 37.5 µm.

The ability of the mutant mice to produce gasping activity in the hypoglossal nerve and diaphragm suggests that their respiratorymotor efferent pathway was functional. Histological examinationshowed that the hypoglossal motor nucleus in the brainstem ofmutant mice was intact (Fig. 8B). It is possible that a defectin the neural control of respiration may result from disruptedrespiratory rhythmogenesis or neurotransmission in the Dnmt1-deficientbrain.

DNA hypomethylation results in rapid cell death in the postnatal brain

The observations described so far suggest that Dnmt1 deletion and subsequent hypomethylation did not affect the survival ofneuronal cells in the prenatal brain, although mutant animalsdied immediately after delivery. We were interested in investigatingthe fate of brain cells in postnatal mutant animals. In the experimentsdescribed above, Dnmt1 had been deleted in ~95% of brain cells(see Fig. 4A,B) by expression of the cre recombinase from a paternallytransmitted nestin-cre transgene crossed with females carryingthe Dnmt1^2lox target allele. However, when the nestin-cre transgene was transmittedmaternally and the Dnmt1^2lox target allele was derived paternally, the recombination frequencywas only 30% instead of 95% in the adult brain, indicating thatthe cre transgene was imprinted and the expression level was dependenton parental origin (compare Figs. 9A and 4A,B). The fraction ofbrain cells that performed the cre-mediated recombination wasalready ~30% at E12 with maternal nestin-cre transmission, andthis fraction did not increase during later development. Thiswas shown by crossing females carrying the nestin-cre transgenewith males carrying a lacZ reporter gene (the Rosa26 reporter;Soriano, 1999), which resulted in ~30% lacZ-positive cells inthe brains of E12, newborn, and adult animals (data not shown).To determine the fraction of Dnmt1 mutant cells in animals carryinga maternally derived nestin-cre transgene and a paternally derivedDnmt1^2lox allele, we performed Southern blot analyses with E12 and newbornbrain tissues. Loop-out frequency was ~30% at E12 (Fig. 9B, lane1) and at birth (Fig. 9A,B), indicating that the fraction of mutantcells did not change during embryonic development. Thus, mutantmice carrying the maternally derived nestin-cre transgene hada mosaic brain in which Dnmt1-deficient (Dnmt1^1lox) and Dnmt1-proficient (Dnmt1^2lox) cells coexisted and Dnmt1-deficient cells were not selectedagainst during the embryonic stages of development.

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Figure 9. Postnatal loss of Dnmt1-deficient brain cells in mutant mice with maternal inheritance of the nestin-cre transgene. A, Southern blot analysis of the Dnmt1 gene deletion in DNA from different brain regions of mutant mice after maternal inheritance of the nestin-cre transgene. At the newborn stage ~30-35% of Dnmt1 gene deletion was detected in both mutant and heterozygous brains. FB, Forebrain; Col, colliculus; CB, cerebellum; BS, brainstem; SP, spinal cord. B, Dnmt1-deficient brain cells are eliminated during postnatal development. Deletion of the Dnmt1 gene was maximal by E12.5 (Br, whole brain) and remained constant in the brain throughout the late stage of embryogenesis and at the postnatal day 1 (P1; also see A). However, only a very small number of cells (4-6%) carrying the Dnmt1 deletion was detected in the cortex (CX) and cerebellum (CB) in 2-week-old (P14) mutant mice. By P21, Dnmt1-deficient cells were not detectable by Southern blot analysis in the cortex, cerebellum, or other regions of the brain (data not shown). mutant, Mutant mice with the Nestin-cre;Dnmt1^2lox/N genotype. con, Control samples from Nestin-cre;Dnmt1^+/2lox mice, which showed constant levels of the Dnmt1 deletion at P1 and P21.

Because newborn mutants with a maternally transmitted cre transgene were born alive and normal, we examined whether Dnmt1-deficientneurons survived postnatally. To assess the survival of Dnmt1-deficientcells, we performed Southern blot analyses to determine the percentageof mutant cells in brain tissues at different postnatal stages.Figure 9B shows that the fraction of brain cells with cre-mediatedDnmt1 deletion in heterozygous mice (Dnmt1^+/2lox carrying the maternally derived nestin-cre transgene) remainedconstant during the first 3 weeks of postnatal development. Incontrast, the frequency of cre-mediated Dnmt1 deletion in mutantmice was initially 30% at the newborn stage but decreased significantlyby P14. At 3 weeks of age Dnmt1-deficient cells were not detectableby Southern blot analysis in either the cerebellum or cortex (Fig.9B) or other brain regions (data not shown). These results indicatethat Dnmt1-deficient neurons were eliminated from the postnatalbrain, in contrast to the prenatal brain in which hypomethylationhas no apparent effect on cellsurvival.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previous work had established that Dnmt1 is highly expressed in embryonic and postnatal neurons of the brain (Goto et al.,1994; Brooks et al., 1996; Trasler et al., 1996; Inano et al.,2000). This finding was surprising, given that the known functionof Dnmt1 is to maintain the parental methylation pattern of thedaughter DNA strands in mitotic cells. Dnmt1 is, therefore, highlyexpressed during S-phase in mitotic cells but is downregulatedin resting cells (Szyf et al., 1991). Because deletion of Dnmt1from the germline causes apoptosis and early embryonic lethality(Li et al., 1992), this mutant line was not useful for studyingthe possible function of DNA methylation in brain development.As a first approach to assessing the role of methylation duringbrain development and postnatal life, we generated a Dnmt1 conditionalallele that can be deleted at postmitotic CNS neurons or E12 CNSprecursor cells. Although Dnmt1 is not essential for maintainingglobal DNA methylation in postmitotic neurons, the enzyme is requiredfor the methylation of mitotic precursor cells and their daughtercells. Hypomethylated CNS cells survived through the late stagesof embryogenesis but died postnatally. In addition, hypomethylationin the brain leads to abnormal neural control of respiration atbirth. These findings indicated that DNA methylation is crucialfor the function and survival of postnatal CNSneurons.

When Dnmt1 gene deletion is mediated by the nestin-cre transgene, Dnmt1 deficiency occurred in the brain at E12.5, a stagewhen neurogenesis is still actively ongoing (Austin and Cepko,1990; Cepko et al., 1990). This suggests that precursor cellsin the embryonic mutant brain are able to generate mature neurons(and non-neuronal cells) in the absence of Dnmt1. The mutant cellsand their mitotic descendants survive for at least another 7 duntil birth, as supported by both in vivo and in vitro evidence.Indeed, the fraction of Dnmt1-deficient cells, either 95% or 30%,depending on the parental origin of the nestin-cre transgene,remained constant in the mutant brain from E12.5 to the newbornstage. Histological examination of mutant fetal brains did notshow any obvious increase in the number of pyknotic nuclei andTUNEL-positive cells, suggesting that DNA hypomethylation didnot increase the rate of neuronal cell death in vivo. These observationsargue that DNA hypomethylation did not confer a selective disadvantageon the survival of the hypomethylated embryonic neurons in vivo.Likewise, the in vitro survival of embryonic cortical neuronsexplanted from mutant brains was indistinguishable from that ofcontrols. Nevertheless, we cannot exclude the possibility that,in the mutant brain, a small fraction of Dnmt1-deficient cellsmay undergo rapid turnover that is below our detectionlevel.

In contrast to the significant demethylation observed in the CNS neurons of Nestin-cre;Dnmt1 mutants, Dnmt1-deficient neuronsin CamK-cre;Dnmt1 conditional mutants were long-lived and didnot show any significant demethylation in the highly methylatedDNA repeats. The difference in DNA methylation between Nestin-cre;Dnmt1and CamK-cre;Dnmt1 mutant cells could be attributable simply tothe fact that only Dnmt1-deficient cells in Nestin-cre;Dnmt1 conditionalmutants undergo mitosis that results in passive DNA demethylation.The stable DNA methylation pattern in Dnmt1-deficient neuronsof CamK-cre;Dnmt1 conditional mutants is not surprising, becausethere is no direct evidence that DNA methylation undergoes anydynamic turnover in normal adult neuronalcells.

The survival of hypomethylated embryonic CNS neurons in Nestin-cre;Dnmt1 conditional knock-outs is in apparent contrast tothe extensive apoptosis observed in the brain of the Dnmt1 mutantembryos just after gastrulation (Li et al., 1992). We considerthe following mutually nonexclusive possibilities: (1) DNA hypomethylationin the Dnmt1 conditional neuronal cells may be less extensivethan in the rapidly dividing non-neuronal cells of the gastrulatingmutant embryos. For example, in Dnmt1 homozygous mutant male embryosectopic Xist gene activation was seen in ~15% of the cells (Panningand Jaenisch, 1996), whereas only 4-8% of brain cells showed ectopicXist transcription after cre-mediated Dnmt1 deletion, perhapsreflecting a less severe genomic demethylation in the neuronsas compared with somatic cells of the postgastrulation Dnmt1 nullembryo. To reach a critical level of hypomethylation, cells haveto undergo several rounds of DNA replication after the deletionof Dnmt. It is possible that the number of cell divisions thatseparate postmitotic neurons from their precursor cells (wherethe cre-mediated Dnmt1 deletion occurs at E9.5-E12) is limited,resulting in less pronounced genomic demethylation in Dnmt1-deficientneurons than in the cells of Dnmt1^/ embryos at the postgastrulation stage. This may lead to lessectopic Xist activation and less pronounced apoptosis. (2) Dnmt3aand 3b are known to be expressed in the developing brain (Okanoet al., 1998), and these enzymes may compensate for the loss ofDnmt1 function in mutant neurons. (3) Finally, it is possiblethat prenatal neurons are intrinsically more resistant to theconsequences of genomic DNA demethylation than the cells of thepostgastrulationembryo.

As an epigenetic factor, DNA methylation patterns may be subject to active regulation in the nervous system in response toparticular stimuli. Endres et al. (2000) recently demonstratedthat levels of DNA methylation activity in the brain actuallyare increased with ischemic injury, and this increase is partlydependent on Dnmt1 activity. Blocking Dnmt1 activities, eithergenetically or pharmacologically, is protective to the injuredneurons, suggesting that a balance of DNA methylation levels isimportant for neuronal survival (Endres et al., 2000). Brookset al. (1996) suggested that Dnmt1 expression in postmitotic neuronsmay serve to maintain DNA methylation after base-excision repairof the G:T mismatch that can occur with deamination of the methylatedcytosine. Recently, Inano et al. (2000) demonstrated that Dnmt1protein in adult CNS neurons is localized primarily in the cytoplasm,raising the possibility that Dnmt1 may play a novel function otherthan DNA methylation in these cells. Fuks et al. (2000) demonstratedthat Dnmt1 itself contains a transcription repression domain thatdirectly recruits histone deacetylases, suggesting an active rolefor Dnmt1 in chromatin remodeling. Furthermore, Dnmt1 is an activecomponent of several repressive transcriptional complexes thatcan directly target transcriptional silencing to particular classesof genes or during the S-phase of the cell cycle (Robertson etal., 2000; Rountree et al., 2000). These findings certainly provideus with the clues to look further into the molecular and cellularchanges in Dnmt1-deficient neurons in Nestin-cre;Dnmt1 and CamK-cre;Dnmt1conditionalmutants.

The lethality of Nestin-cre;Dnmt1 mutant animals appears to be caused by respiratory failure. These mutant animals never initiatedbreathing and showed highly impaired spontaneous neuronal activityrecorded from the 12th cranial nerve. The neural mechanism underlyingthis defect is still unclear. It is possible that genomic hypomethylationalters the expression pattern of genes that are involved eitherdirectly or indirectly in respiratory control and thus interfereswith the initiation of normal breathing. It is of interest tonote that mutations of a methyl-binding protein MECP2 have beenassociated with the neurodevelopmental disease Rett syndrome (Amiret al., 1999) in which the patients often exhibit respirationirregularities in addition to behavioral defects and mental retardation(Kerr, 1992; Naidu, 1997; Armstrong et al., 1999). Because a majorfunction of the MECP2 protein is to mediate methylation-inducedgene silencing, it is possible that the phenotype of DNA hypomethylationin the postnatal brain may overlap partially with what is observedin MECP2 deficiency. Understanding the role of DNA methylationin brain development and function at the molecular level alsomay shed light on the disease mechanisms in Rettsyndrome.

  FOOTNOTES

Received Aug. 14, 2000; revised Oct. 30, 2000; accepted Nov. 2, 2000.

This work was supported by National Institutes of Health Grants R35 CA44339 (to R.J.), HL52925 and HL60064 (to C.S.P.), HD18184(to C.B.W.), and CA44338 (to J. M. Bishop). Financial supportalso comes from a Medical Foundation postdoctoral fellowship (G.F.),from a National Institutes of Health postdoctoral fellowship (R.Z.C.),and from the Deutsche Forschungsgemeinschaft (A.T.). We thankJessie Dausman, Ruth Flannery, and Jeanne Reis for technicalsupport.
Correspondence should be addressed to Dr. Rudolf Jaenisch, Whitehead Institute for Biomedical Research, Nine Cambridge Center,Cambridge, MA 02142. E-mail: jaenisch{at}wi.mit.edu.

Dr. Bates's present address: Genetics Institute, Cambridge, MA02140.

Dr. Lee's present address: Department of Biology, University of California, San Diego, La Jolla, CA92093.

Dr. Kühn's present address: Artemis Pharmaceuticals, Cologne,Germany.

Dr. Trumpp's present address: Swiss Institute for Experimental Cancer Research, CH-1066 Epalinges,Switzerland.

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