Neuronal Expression of Zinc Finger Transcription Factor REST/NRSF/XBR Gene

QUICK SEARCH:

[advanced]

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

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

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 (130)

Citing Articles via Google Scholar

Google Scholar

Articles by Palm, K.

Articles by Timmusk, T o.

Search for Related Content

PubMed

PubMed Citation

Articles by Palm, K.

Articles by Timmusk, T o.

Pubmed/NCBI databases
Gene GEO Profiles
HomoloGene Nucleotide
Protein UniGene
Compound via MeSH
Substance via MeSH

Previous Article  |  Next Article

The Journal of Neuroscience, February 15, 1998, 18(4):1280-1296

Neuronal Expression of Zinc Finger Transcription Factor REST/NRSF/XBR Gene
Kaia Palm¹, Natale Belluardo², Madis Metsis¹^,³, and T õnis Timmusk¹^,⁴
¹ Laboratory of Molecular Neurobiology, Department of Medical Biochemistry and Biophysics, Karolinska Institute, S-171 77 Stockholm, Sweden, ² Institute of Human Physiology, Faculty of Medicine, University of Catania, I-95125 Catania, Italy, ³ Gene Technology Center, Tallinn, EE0026 Estonia, and ⁴ Department of Developmental Neuroscience, Biomedical Center, Uppsala University, S-751 23 Uppsala, Sweden

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The identification of a common cis-acting silencer element, a neuron-restrictive silencer element (NRSE), in multiple neuron-specificgenes, together with the finding that zinc finger transcriptionfactor REST/NRSF/XBR could confer NRSE-mediated silencing in non-neuronalcells, suggested that REST/NRSF/XBR is a master negative regulatorof neurogenesis. Here we show that, although REST/NRSF/XBR expressiondecreases during neuronal development, it proceeds in the adultnervous system. In situ hybridization analysis revealed neuronalexpression of rat REST/NRSF/XBR mRNA in adult brain, with thehighest levels in the neurons of hippocampus, pons/medulla, andmidbrain. The glutamate analog kainic acid increased REST/NRSF/XBRmRNA levels in various hippocampal and cortical neurons in vivo,suggesting that REST/NRSF/XBR has a role in neuronal activity-impliedprocesses. Several alternatively spliced REST/NRSF/XBR mRNAs encodingproteins with nine, five, or four zinc finger motifs are transcribedfrom REST/NRSF/XBR gene. Two of these transcripts are generatedby neuron-specific splicing of a 28-bp-long exon. Rat REST/NRSF/XBRprotein isoforms differ in their DNA binding specificities; however,all mediate repression in transient expression assays. Our datasuggest that REST/NRSF/XBR is a negative regulator rather thana transcriptional silencer of neuronal gene expression and counteractswith positive regulators to modulate target gene expression quantitativelyin different cell types, including neurons.

Key words: REST; NRSF; XBR; transcription factor; zinc finger; silencer; negative regulator; repressor; gene structure; neuron-specific splicing; neuronal expression; brain; kainic acid; NRSE; BDNF

  INTRODUCTION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The balance between negative and positive regulators is critical in determining cell type and developmental stage-specifictranscription of a gene. Recently, two groups identified a geneencoding zinc finger protein that was suggested to function asa master regulator of the neuronal phenotype. Transcription factorREST, an RE1-silencing transcription factor (Chong et al., 1995),also known as neuron-restrictive silencer factor (NRSF; Schoenherrand Anderson, 1995a) was identified as a factor that could interactwith a 23 bp cis-element, a neuron-restrictive silencer element(NRSE/RE1), and mediate silencing of type II voltage-dependentsodium channel (NaCh II) and SCG10 genes in non-neuronal cells.Analysis of the REST/NRSF mRNA expression pattern, exclusive tothe CNS neurons, together with the results of transient expressionassays, suggested that REST/NRSF acts as a silencer of neuron-specificgene expression in the undifferentiated neuronal progenitors andin non-neuronal cells (Chong et al., 1995; Schoenherr and Anderson,1995a). Since then, several other neuronal genes that contributeto many different aspects of neuronal phenotype have been shownto contain functional NRSE-like sequences in their regulatoryregions (Schoenherr et al., 1996). However, some of the publisheddata do not support the proposed role of REST/NRSF/XBR as a neuron-restrictivesilencer factor. For example, the same factor has been identifiedas an X2 box repressor (XBR), which represses the promoter activityof DPA, the immune system-specific major histocompatibility complexclass II gene in terminally differentiated B-cell lineage (Schollet al., 1996). This suggested that REST/NRSF/XBR-mediated repressionis not limited to genes involved in neuron-specific functions.It also has been reported that brain-derived nuclear extractscontain NRSE binding proteins (Thiel et al., 1994). Recently,with the use of transgenic mice, it was demonstrated that NRSEis involved in the repression of neuronal nicotinic acetylcholinereceptor $beta$ 2-subunit promoter activity in the neurons of adultbrain (Bessis et al., 1997).

Data indicating that NRSE binding proteins regulate transcription in neurons have led us to study the expression and presenceof REST/NRSF/XBR or its putative neuronal homologs in the adultbrain. We show that multiple rat REST (rREST) transcripts areexpressed in the neurons of adult brain, and we characterize themolecular basis for these alternatively spliced transcripts bystructural analysis of the rREST gene. We further show that theexpression of different rREST transcripts is increased in thebrain after kainic acid (KA)-induced seizures, and we analyzethe potential role of rREST and its protein isoforms by usingfunctional assays. Our data suggest that REST/NRSF/XBR is involvedin the modulation of the target gene expression in the matureneurons.

  MATERIALS AND METHODS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Isolation and characterization of cDNA clones. A randomly primed cDNA library was constructed in $lambda$ ZAPII vector from RN33Bcell poly(A⁺) mRNA (kindly provided by Dr. C. F. Ibañéz, Karolinska Institute)with the cDNA synthesis kit (Stratagene, La Jolla, CA) and screenedat low-stringency conditions with the full-length human REST/NRSF/XBRcDNA (kindly provided by Dr. G. Mandel, State University of NewYork at Stony Brook). One of the positive clones contained a cDNAfragment of ~2.5 kb. Restriction fragments of this rREST cDNAclone PvuII/PstI (encompassing zinc fingers 2-8) and PstI/SacI(encoding a part of the finger 8 and the region immediately downstream)were applied in the subsequent screenings of the same library.DNA fragments used as hybridization probes were labeled radioactivelywith [ $alpha$ -³²P]dCTP by random priming (Feinberg and Vogelstein, 1983) to aspecific activity of ~10⁹ cpm/µg. Positively hybridizing phages were isolated, appliedto in vivo excision, and analyzed by DNA sequencing (T7 sequencingkit, Pharmacia, Uppsala, Sweden). Sequence comparison was performedwith a software package of the University of Wisconsin GeneticsComputer Group (Devereux et al., 1984).

Southern blot analysis. High-molecular-weight Sprague Dawley rat chromosomal DNA (20 µg) was digested with EcoRI and BamHI.The fragments were separated in 1.0% agarose gel and transferredto Hybond N⁺ filter (Amersham, Braunschweig, Germany). Then the filter washybridized with the [ $alpha$ -³²P]dCTP-labeled rREST cDNA fragment from riboprobes 4 and 5 (describedin RNase Protection Analysis). At first the filter was washedwith 2× SSC, 0.1% SDS at 50°C, and imaged. After initial imaging,the filter was washed with 0.2× SSC, 0.1%SDS at 65°C, and reexposed.The filters were imaged with PhosphorImager, and the digitizedimages were analyzed with ImageQuant software (Molecular Dynamics,Sunnyvale, CA).

RNA preparation and Northern blot analysis. Total and poly(A⁺) RNA from indicated tissues and cell lines were purified andanalyzed by Northern blot as described (Timmusk et al., 1993).The filters were hybridized with the same rREST cDNA fragmentsas in the rescreening of the RN33B cDNA library.

RNase protection analysis. RNase protection assays (RPA) were performed with the RPAII Ribonuclease Protection Assay Kit (Ambion,Austin, TX). The templates used to generate cRNA probes were clonedin pBSKS vector (Stratagene), linearized in the 5' end, and transcribedwith T7 or T3 RNA polymerase (Promega, Madison, WI). The rREST-specificriboprobes that were applied included the following: (1) for 5'-untranslatedregion (5'-UTR) of type A, a 270 bp EcoRI/PvuII fragment of rREST13cDNA; (2) for 5'-UTR of type B, a 260 bp EcoRI/PvuII fragmentof rREST16 cDNA; (3) for 5'-UTR of type C, a 330 bp EcoRI/PvuIIfragment of rREST11 cDNA. The 5'-UTR-specific probes yielded afully protected fragment corresponding to the 5'-UTR-specifictranscript and a 190 bp fragment corresponding to all other rRESTtranscripts; (4) a 460 bp PvuII/AvaII fragment, including theregion upstream of zinc finger 1 up to zinc finger 2; (5) a 360bp AvaII/DraI fragment, spanning the region between zinc fingers2 and 6; (6) for the truncated rREST1, a 370 bp AvaII/HindIIIfragment of rREST1 cDNA. This probe yielded a fully protectedfragment corresponding to rREST1 mRNA and a 256 bp fragment correspondingto all other rREST transcripts; (7) for rREST2 respective reversetranscription (RT)-PCR cDNA fragment spanning the region fromzinc finger 2 to zinc finger 8 (8) for rREST3, (9) for rREST4and (10) for rREST5, respective RT-PCR cDNAs covering the regionfrom zinc finger 5 to zinc finger 8; (11) a 360 bp XhoI fragmentof rREST38 cDNA, covering the region upstream of zinc finger 9.For determining the levels of mouse REST/NRSF/XBR mRNA in Neuro-2Acells, a 380 bp HaeIII fragment of mouse REST/NRSF/XBR cDNA (GenBankaccession number U13878), covering the region from zinc finger2 to zinc finger 6, was cloned in pBSKS and used as a templatefor in vitro transcription. The quantification of the REST mRNAabsolute amounts in tissues and cell lines was performed as described(Timmusk et al., 1994). Briefly, for quantification of rat andmouse REST/NRSF/XBR mRNAs, standard curves were constructed withknown amounts of in vitro synthesized, unlabeled sense strandREST RNA hybridized with the excess of labeled antisense probe.The sense strand transcript was made by linearizing the same DNAtemplate as that used for antisense probe synthesis on the oppositeside of the probe insert. Then in vitro transcription with T3or T7 RNA polymerase was used to synthesize the unlabeled sensestrand. The absolute amount of sense RNA that was synthesizedwas measured spectrophotometrically. Samples containing 20 µgof total RNA from embryonic day 13 (E13) brain, E16 heart andlung, E19 kidney, adult rat brain and thymus, and Neuro-2A andC6 cells were analyzed in parallel with the samples used to generatethe standard curve. Quantification of the amount of REST-specificmRNA that hybridized to the probe in different tissue sampleswas performed with PhosphorImager, using ImageQuant software (MolecularDynamics).

PCR analysis of rREST mRNA expression and gene structure. First-strand cDNAs were synthesized with reverse transcriptase (SuperscriptII, Life Technologies, Gaithersburg, MD), using 5 µg of poly(A⁺) RNA from different tissues as a template and oligo-dT (Promega)as a primer. PCR reactions were performed in a volume of 25 µlcontaining one-tenth of RT reaction as a template and 0.25 U ofthermostable DNA polymerase (Dynazyme, Finnzymes, Finland). DNAwas amplified with PTC-100 TM thermocycler (MJ Research, Watertown,MA) at the following conditions: 94°C (2 min), 35 cycles of 94°C(40 sec), 60°C (40 sec), and 72°C (150 sec). To detect rREST 5'-UTR-specifictranscripts, we increased the number of cycles to 45. The amplifiedRT-PCR products were analyzed on 2% agarose gel.

Amplification of genomic DNA by PCR was performed by using the Expand Long Distance PCR System kit (Boehringer Mannheim, Mannheim,Germany) according to manufacturer's instructions. Annealing temperaturewas 60°C for all combinations of primers, and the number of cycleswas 35. Primers (Eurogentec, Brussels, Belgium) that were appliedincluded the following: pA^s, 5'-GGC AAC AAA GAA AAG GAG TTA GAG CGA-3'; pB^s, 5'-GCG GAG CCC CGG TAC AGG CCC GAT-3'; pB^as, 5'-CGT CCG ATC GGG CCT GTA CCG GGG CT-3'; pC^s, 5'-GGA GAA ACG TGG ACA TTC CTT GGA-3'; pATG^s, 5'-GCT ACA GTT ATG GCC ACC CAG GTG AT-3'; pATG^as, 5'-CCA TGC CCA TGT TGC CAC TGT T-3'; p2^s, 5'-CTA CAT GGC ACA CCT GAA GCA CCA C-3'; pR1^s, 5'-CCG TTT CCC AAG GGA ATT GAG GGC T-3'; pR1^as, 5'-GCC CTC AAT TCC CTT GGG AAA CGG TA-3'; p5^s, 5'-GAC TCA TCT AAC TCG ACA CAT GCG T-3'; p5^as, 5'-GCA TGT GTC GAG TTA GAT GAG TCT T-3'; pR4^s, 5'-CAG AGT GTG ATC TAG YTG GGT GA-3'; pR4^as, 5'-GGC TTC TCA CCC ARC TAG ATC ACA CT-3'; pR5^as, 5'-GGC TTC TCA CCT GAA TAC ATA CCC A-3'; pR2^s, 5'-GAC ACA TGC GTA CTC ACT CAG GTT GGT-3'; pR3^s, 5'-CGA CAC ATG CGT ACT CAC TCA GCC ATT-3'; p6^s, 5'-GAC CCG ACA CGC AAG ACA GGT TCA CA-3'; p6^as, 5'-GTG TCG GGT CAC TTC GTG CTG ATT-3'; p8^as, 5'-GCG TAG TCA CAC ACG GGG CAG TTG AAC-3'; and p9^as, 5'-CCA AAT GGC GAT TGA GGT GTT TGC-3', where A, B, and C denotethe different 5'-UTRs; ATG is the translation initiation codon;single numbers 2-9 are the zinc finger motifs 2, 5, 6, 8, and9; R1-R5 are rREST1-, rREST2-, rREST3-, rREST4-, and rREST5-specifictranscripts; s is the sense strand; and as is the antisense strand.

Rat genomic DNA (250 or 500 ng) was used as a template for amplifications. Genomic PCR products were cloned into the pMOS^BlueT vector and sequenced by the DNA sequencing system (AB, Perkin-Elmer,Emeryville, CA).

Pharmacological treatments. Adult male Sprague Dawley rats (body weight, 200-230 gm; Alab, Stockholm, Sweden) were used inall experiments. KA (0.35 µg/0.5 µl) or saline as a control wasinjected bilaterally in the brain lateral ventricle (Salin etal., 1995), and the animals were killed at the indicated timesafter the injections. All animal experiments were approved bythe local ethical committee.

In situ hybridization. Serial coronal sections (14 µm) from fresh frozen adult rat brain were analyzed by in situ hybridizationas described (Timmusk et al., 1993; Belluardo et al., 1997). Twodifferent [ $alpha$ -³⁵S]-labeled rREST cRNA probes were applied (riboprobes 4 and 11;described in RNase Protection Analysis and Fig. 1B). The hybridizationspecificity was confirmed by using [ $alpha$ -³⁵S]-labeled sense riboprobes synthesized from the same templates.Both sense probes resulted in the hybridization signal equivalentto the background. Emulsion-dipped sections were developed after6 weeks by using D-18 developer (Kodak, Rochester, NY), fixed,and counterstained with cresyl violet. Staining of the brain sectionsallowed us to distinguish large and weakly stained cells fromsmall and strongly stained cells. The relative levels of rRESTmRNA expression per cells were evaluated by counting the numberof silver grains over individual cells with a computer-assistedimage analysis system (IBAS I-II, Zeiss, Kontron, Munich, Germany).A correction factor for overlapping grains was applied. Labeledcells were defined on the basis that they showed more than fivesilver grains, as compared with the background, which was calculatedby counting the grains around and close to labeled cells. Dataare presented in an arbitrary semi-quantitative scale of labelingintensity. "Low intensity of labeling" (±) defined the amountof silver grains between the fixed minimum level and 10 grainsper cell; "moderate intensity of labeling" (+) defined the numberof grains between 10 and 20; " high intensity of labeling" (++)defined the number of grains exceeding the maximum level selectedfor the moderate intensity.

Cell culture, DNA transfection, and CAT assays. Mouse Neuro-2A and rat C6 cell lines were grown in DMEM supplemented with10% fetal bovine serum. Primary cell cultures of hippocampal andcortical neurons and astrocytes were prepared as described earlier(O'Malley et al., 1994). For transfection experiments the followingDNA constructs were made. MseI/ScrFI fragment located at 1873-1964bp within BDNF promoter II region and containing the palindromicNRSE sequence (Timmusk et al., 1993) was cloned into pBLtkCATvector (Luckow and Schutz, 1987; Jacoby et al., 1989) upstreamof the thymidine kinase promoter (pNRSE^BDNFCAT) into SalI site. rREST expression deletion mutants rREST402D,rREST2-5^trunc, and rREST1^trunc are original cDNA clones from the second screening that werecloned into pcDNA3 (Invitrogen, San Diego, CA). Neuro-2A and C6cell lines were transfected by the calcium phosphate precipitationmethod, as described previously (Timmusk et al., 1993; Chiaramelloet al., 1995). Freeze-thaw lysates of cells collected 48 hr afterthe transfection were assayed for CAT activity as described (Pothieret al., 1992). At least two different DNA preparations were testedfor each plasmid. To normalize the transfection efficiencies,we cotransfected cells with pON260 expressing $beta$ -galactosidase(Spaete and Mocarski, 1985). Quantification of the acetylatedratios was performed with PhosphorImager, using ImageQuant software(Molecular Dynamics). All CAT activities were normalized to totalprotein and $beta$ -galactosidase activity.

Electrophoretic mobility shift assay. Recombinant proteins of rREST and rREST deletion mutants were produced by coupled invitro transcription and translation with a rabbit reticulocytelysate according to the manufacturer's protocol (Promega). Thefollowing oligonucleotides, NRSE1^s, 5'-GGCGAGCAGAGTCCATTCAGCACCTTGGACAGAGCCAGCGG-3'; NRSE1^as, 5'-CCGCTGGCTCTGTCCAAGGTGCTGAA-3'; NRSE2^s, 5'-CAGCCAGCGGATTTGTCCGAGGTGGT-3'; and NRSE2^as, 5'-CCTGGATGAAGTACTACCACCTCGGACAAATCCGCTGGCTC-3', correspondingto the upper and lower half sites of NRSE^bdnf palindrome, were synthesized (Eurogentec) as paired sense andantisense oligonucleotides, annealed, and filled at their 3' recessedends, using Klenow enzyme (United States Biochemicals, Cleveland,OH) to create double-stranded unlabeled specific competitors NRSE11and NRSE21. To prepare [ $alpha$ -³²P]dCTP-labeled NRSE^bdnf probe, we cleaved the pNRSE^BDNFCAT plasmid with HindIII/XbaI and labeled it with Klenow enzyme(United States Biochemicals). Mobility shift assays were performedas described (Chiaramello et al., 1995).

  RESULTS

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Cloning of rat zinc finger transcription factor REST/NRSF/XBR (rREST)

A randomly primed cDNA library prepared from poly(A⁺) RNA of the rat Raphe nucleus-derived cell line (RN33B) (Whittemore andWhite, 1993) was screened at low stringency with the human REST/NRSF/XBRfull-length cDNA (Chong et al., 1995). Sequence analysis revealedthat the isolated cDNA clones showed a high degree of sequencesimilarity with the human REST/NRSF/XBR cDNA in the zinc fingercluster region and apparently encoded the rat homolog of REST/NRSF/XBR(rREST). Several clones differed in their 5' sequences upstreamof the first ATG, defined by analogy to the human REST/NRSF/XBRtranslation initiation sequence. Altogether, three different 5'-UTRswere identified (designated as types A, B, and C). A majorityof the clones shared type A 5'-UTR that showed some homology tothe human NRSF cDNA 5' region (GenBank accession number U13879).Three cDNA clones shared type B 5'-UTR of various lengths. Oneclone contained the type C 5'-UTR, presumably referring to therare use of this type 5'-UTR. All of the different 5' regionsextended the open reading frame (ORF) by 9 bp, preceded by thetermination codon and 5'-UTRs of various lengths. A combinationof the sequences of several rREST cDNAs formed an ORF that predicteda protein of 1083 amino acids with nine zinc finger motifs (Fig.1). However, one of the clones, rREST1, showed an in-frame terminationcodon immediately after the region encoding zinc finger 4, predictinga truncated form of rREST protein with four zinc fingers. A searchof the GenBank expressed sequence tags (EST) database revealedthat a human EST sequence (GenBank accession number U13877)differs from the human REST/NRSF/XBR cDNA sequence precisely inthe same nucleotide position as rREST1 cDNA from the full-lengthrREST cDNA (Fig. 1A). This finding suggested a general mechanismof REST/NRSF/XBR gene regulation that is conserved across species.

View larger version (73K):
[in this window]
[in a new window]
Figure 1. Primary structure of rREST cDNA and the predicted rREST protein. A, Optimized alignment of the rREST and human REST/NRSF/XBRamino acid sequences. Vertical lines indicate identical aminoacid residues. Zinc fingers are boxed. Y marks the divergenceof rREST from rREST1^trunc and rREST2-5^trunc. Stop codons are indicated by an asterisk. B, Schematic representationof rREST full-length cDNA encoding rREST protein with nine zincfinger motifs. Zinc finger motifs are shown as vertical gray bars.The long unfilled box indicates ORF. 5'- and 3'-UTR regions areindicated as thick lines. cRNA probes used in Southern analysis,RNase protection assays, and in situ hybridization are shown belowin relation to the rREST cDNA. Thin lines in the cRNA probes correspondto the unique parts of respective rREST transcripts. R., Rat;H., human. The nucleotide sequences of rREST cDNAs have been submittedto GenBank under accession numbers AF 037199, AF 037200, AF 037201,AF 037202, and AF 037203.

The deduced amino acid sequence of rREST, as compared with the human REST/NRSF/XBR protein sequence, is shown in Figure 1A.The ORF of rREST is overall 75% identical with the ORF of thehuman REST/NRSF/XBR at the nucleic acid level. At the amino acidlevel these two proteins share 70% identity. Like the human REST/NRSF/XBR,rREST gene encodes a protein with the cluster of eight zinc fingermotifs located in the N terminus and a distinct ninth zinc fingermotif in the C terminus. Zinc finger motifs of REST/NRSF/XBR arehighly conserved between rat and human, the difference being infew, albeit nonconserved, amino acid substitutions in the fingermotifs 4 and 5. Zinc finger motifs of the rREST and mouse REST/NRSF/XBR(GenBank accession number U13878) proteins are 100% conserved.Sequence analysis of the region separating the N- and C-terminalzinc finger clusters of rREST reveals 67% identity at the nucleicacid level and 54% identity at the amino acid level, as comparedwith the corresponding area in human REST/NRSF/XBR. This regionshows a high proportion of proline and acidic amino acid residuesbut no repetitive proline-enriched motifs, characteristic forthe human REST/NRSF/XBR. The differences in the secondary structureof the proline-rich region between species could be compensatedby similar higher order structural folding if this region in humanREST/NRSF/XBR and rREST proteins forms a functionally conservedinteraction surface. Protein divergence between species is quitecommon to the family of zinc finger transcription factors, reflectingthe process of evolution from a common ancestor. The human andmouse Krüppel-like ortholog (MOK-2) genes present one of themost extreme examples of the process of evolutionary divergence.These genes encode functionally different zinc finger transcriptionfactors attributable to the loss of part of the gene that correspondsto the activator domain in the mouse MOK-2 protein (Ernoult-Langeet al., 1995).

Putative PEST-like sequences that have been found in proteins destined to rapid degradation, with intracellular half-livesof less than 2 hr (e.g., transcription factors E1A, c-myc, p53,c-fos, and v-myb) (Rogers and Rechsteiner, 1986; Rechsteiner andRogers, 1996), are identifiable throughout the rREST protein.The most distinct PEST sequence is located between the amino acids668 and 727 in the proline-enriched region with a PEST-FIND scoreof +16.4, which is considered a significant value to denote theregion of proteolytic targeting (Rechsteiner and Rogers, 1996).This feature strongly suggests that rREST as a transcription factormay have rapid turnover, and/or its activity may be post-translationallyregulated by proteolysis.

REST/NRSF/XBR mRNA is expressed in the neurons of adult rat brain

According to previously reported data, REST/NRSF/XBR mRNA is expressed in most non-neuronal tissues throughout development(Chong et al., 1995; Schoenherr and Anderson, 1995a; Scholl etal., 1996), whereas in the nervous system the expression is restrictedto defined populations of undifferentiated neuronal progenitors(Chong et al., 1995; Schoenherr and Anderson, 1995a). Our Northernblot analysis confirmed the earlier findings showing that rRESTmRNA levels decrease during brain development. However, we alsocould detect the expression of rREST gene in adult rat CNS. rRESTtranscript of 7-8 kb was present at variable levels in spinalcord and all brain regions studied (e.g., striatum, thalamus/hypothalamus,pons/medulla, hippocampus, cerebellum, midbrain, septum, olfactorybulb, cerebral cortex, and colliculi) (Fig. 2).

View larger version (92K):
[in this window]
[in a new window]
Figure 2. Northern blot analysis of rREST mRNA expression. Poly(A⁺) RNA (10 µg) isolated from the indicated rat brain regions, peripheraltissues, and rat C6 glioma cells was electrophoresed in the agarosegel, transferred to Hybond N⁺ filter, and hybridized to the rREST cDNA fragment covering theregion between zinc finger motifs 2 and 8. A, rREST mRNA expressionin various regions of adult rat brain and in rat C6 glioma cells.B, rREST mRNA expression in non-neuronal tissues (testis, spleen,and muscle) and during the development of brain and spinal cord.The position of rREST mRNA-specific signal and migration of 28Sribosomal RNA are indicated. Integrity of RNAs was checked byreprobing the blot with a GAPDH cDNA probe. C6, Rat C6 gliomacell line; str, striatum; thal, thalamus; p/m, pons/medulla; hc,hippocampus; cblm, cerebellum; v midbr, ventral midbrain; sept,septum; o bulb, olfactory bulb; ctx, cerebral cortex; coll, colliculi;spc, spinal cord; E, embryonic day; P, postnatal day; ad, adult.

In situ hybridization was used to study the cellular localization of rREST mRNA expression in the adult rat brain. Hybridizationwith two different cRNA probes (see Materials and Methods andFig. 1B) resulted in identical labeling. Widespread expressionof rREST mRNA was observed in cells displaying neuronal profile(large cells with weakly stained nuclei) (Table 1; Figs. 3, 4).In the olfactory system, diffuse labeling was seen in the granulecell layer (Fig. 4A) and in the plexiform layers. The cerebralcortex showed labeled neurons in all cortical layers (Figs. 3C,4C). In the hippocampal formation the granular neurons in thedentate gyrus and the neurons of the pyramidal layers were labeled(Figs. 3D, 4B,D). In the basal ganglia the regions of the caudateputamen, the globus pallidus, and the accumbens showed no rREST-specificsignal. In the septum and basal forebrain only very few labeledcells were observed. Labeled cells were found over the hypothalamicnuclei and the nuclei of the preoptic area. rREST mRNA was foundto be expressed in most of the thalamic nuclei, particularly inthe dorsal nuclei (Fig. 3E). In the mesencephalon the neuronsof the substantia nigra pars compacta (Figs. 3F, 4G) and the neuronsof the ventral tegmental area and of the red nucleus (Fig. 3G)were found to be positive for rREST mRNA, whereas tegmentum andtectum showed diffuse labeling. In the cerebellar cortex rREST-specificsignal was seen over the granular cell layers, with distinct labelingin the cells along the border between the granular and molecularlayers (Figs. 3H, 4E). Scattered cells were labeled in the molecularlayer of cerebellum. The deep cerebellar nuclei also showed labeledcells (Fig. 3I). rREST signal-positive cells were found in mostnuclei of pons, like the pontine nuclei (Fig. 3J), nucleus trapezoidbody (Fig. 3K), and in the reticular nuclei (Fig. 4F). rREST mRNA-specificsignal was seen virtually in all of the nuclei of the myelencephalon.


View this table:
[in this window]
[in a new window]
Table 1. rREST mRNA expression in the adult rat brain

View larger version (163K):
[in this window]
[in a new window]
Figure 3. In situ hybridization analysis of rREST mRNA expression in the adult rat brain. Shown are dark-field emulsion autoradiographsobtained after hybridization of coronal sections of adult ratbrain with the [ $alpha$ -³⁵S]-labeled rREST cRNA probe corresponding to the region upstreamof zinc finger 9 (riboprobe 11; see Materials and Methods andFig. 1B). rREST mRNA-specific labeling is shown in A, olfactorybulb; B, piriform cortex; C, cerebral cortex; D, hippocampus;E, paraventricular nucleus of thalamus; F, ventral midbrain; G,red nucleus; H, cerebellar cortex; I, deep cerebellar nuclei;J, pontine nuclei; and K, nucleus trapezoid body. L, Section ofbrain area shown in H hybridized with sense RNA probe. Exposuretime was 6 weeks. ON, Olfactory nerve layer; Gl, glomerular layer;Pir, piriform cortex; CTX, cerebral cortex; CA1, CA1 region ofthe hippocampus; dg, dentate gyrus of the hippocampus; hi, hilarregion of the dentate gyrus; PVA, paraventricular thalamus nucleusanterior; VTA, ventral tegmental area; SNC, substantia nigra compacta;SNR, substantia nigra reticular; RMC, red nucleus magnocellular;mol and gr, molecular and granular layers of the cerebellar cortex;Med, medial cerebellar nucleus; Pn, pontine nuclei; Tz, nucleustrapezoid body; ml, medial lemniscus. Arrowheads in H indicatelabeled cells along the border between the granular and molecularlayers of cerebellar cortex. Scale bar: 200 µm in C, E, F, L;100 µm in A, B, D, G, H, I-K.

View larger version (78K):
[in this window]
[in a new window]
Figure 4. Cellular localization of rREST mRNA in the adult rat brain by in situ hybridization. Shown are bright-field emulsion autoradiographsobtained after hybridization of coronal sections of adult ratbrain with the [ $alpha$ -³⁵S]-labeled rREST cRNA probe corresponding to the region upstreamof zinc finger 9 (riboprobe 11; see Materials and Methods andFig. 1B). Shown is rREST-specific labeling in the cells of thefollowing: A, granular layer of olfactory bulb; B, dentate gyrusof hippocampus; C, cerebral cortex; D, CA1 pyramidal layer ofhippocampus; E, along the border between the granular and molecularlayers of the cerebellar cortex; F, gigantocellular reticularnucleus; and G, substantia nigra pars compacta. A section hybridizedwith the sense RNA probe is shown in H, corresponding to the brainarea shown in F. Exposure time was 6 weeks. Arrows point to denseaccumulations of silver grains over individual cells. Scale bar,12 µm.

rREST mRNA was not detected in the cells with glial profile (small cells with strongly stained nuclei), with the exceptionof the olfactory nerve layer (Fig. 3A), which contains only theaxons of olfactory neurons and glial cells. In the non-neuralcells of brain the choroid plexus showed high intensity of labelingfor rREST mRNA. The ependymal cells and meningeal cells (pialcells) also exhibited intense signal (Table 1).

Alternative REST/NRSF/XBR transcripts show different levels of abundance in adult rat brain

We determined the levels of rREST mRNA at different stages of development in various tissues, using quantitative RNase protectionassay (RPA; see Materials and Methods and Fig. 5A). Based on thesedata, the levels of rREST mRNA are highest at the embryonic stagesand decrease continually with age; however, the extent of thedecrease is different in brain, as compared to non-neuronal tissues.Comparison of the levels of rREST mRNA at the embryonic stageswith those seen in adult revealed a fivefold decrease in brainin contrast to a twofold decrease in lung, kidney, and heart.In absolute amounts each cell expresses ~100 molecules of rRESTmRNA in E13 brain, in E16 heart and lung, and in E19 kidney. Inadult heart, lung, and kidney the amount of rREST transcriptshas decreased to ~50 molecules per cell. In the adult rat thehighest levels of rREST mRNA were found in thymus, which expresses~200 rREST transcripts per cell. Quantification revealed thatin the adult brain each cell expresses ~20 molecules of rRESTmRNA, which is 10 times less than in adult thymus or 2.5 timesless than in the adult heart, lung, and kidney. For comparison,the levels of brain-derived neurotrophic factor (BDNF) mRNA transcribedfrom the NRSE-containing promoter II are ~35 molecules per cellin the adult brain (Timmusk et al., 1994). This shows that a potentialtarget gene of rREST is expressed at levels similar to rREST inthe brain.

View larger version (83K):
[in this window]
[in a new window]
Figure 5. Analysis of rREST mRNA expression by RNase protection assay. A, Expression of rREST1 mRNA and all other rREST transcripts(denoted as rREST) in rat brain, in peripheral tissues, and incultured hippocampal and cortical neurons. B, Expression of rRESTtranscripts with 5'-UTRs of type A (panel one), B (panel two),and C (panel three) during rat brain development and in peripheraltissues. C, Top panel, Expression of rREST transcripts exhibitingalternative splicing in the region spanning zinc fingers 5 and6. The arrow indicates the protected fragment that consists ofa mixed population of transcripts rREST2, rREST3, rREST4, andrREST5. Middle panel, Expression of rREST4 mRNA, as compared withthe expression of all other rREST transcripts (denoted as rREST).All bottom panels of A, B, and C show the levels of GAPDH mRNAin the RNA samples that were analyzed. Total cellular RNA (20µg in A and B; 40 µg in C) from each tissue or cultured primaryneurons was analyzed by RPA. The cRNA probes that were used includethe following (see Materials and Methods and Fig. 1B). A, rREST1cDNA fragment encompassing zinc finger motifs 2-4 and the unique3'-UTR of rREST1 cDNA (riboprobe 6). B, First panel, rREST cDNAfragment with type A (riboprobe 1); second panel, type B; thirdpanel, type C (riboprobe 3) 5'-UTRs. C, First panel, rREST cDNAfragment spanning the region between zinc finger motifs 2 and6 (riboprobe 5); second panel, rat REST4-specific cDNA fragment(riboprobe 9). Specific protected fragments are indicated on theleft of each panel. E, Embryonic day; P, postnatal day; ad, adult;H, heart; K, kidney; L, lung; ctx, cerebral cortex; E17 hc, culturedhippocampal neurons; E16 ctx, cultured cortical neurons; ch plex,choroid plexus; astrocytes, cultured hippocampal astrocytes; tRNA,yeast tRNA as a negative control; B+C, mixed population of rRESTtranscripts with 5'-UTRs of types B and C; A+C, mixed populationof rREST transcripts with 5'-UTRs of types A and C; A+B, mixedpopulation of rREST transcripts with 5'-UTRs of types A and B.

We also examined the relative amount of each of the alternative splice variants in the composite pattern of rREST mRNA expression.First, we examined the possibility of tissue-specific expressionof rREST transcripts with three different 5'-UTRs. Assessmentof mRNA levels by RPA analysis revealed that rREST transcriptswith type A 5'-UTR were most abundant (~80% of all of the transcripts)and with type C 5'-UTR were least abundant (~1% of all of thetranscripts) in all analyzed tissues, including brain. AlthoughFigure 5B depicts only a few examples from the variety of tissuesanalyzed, we could not detect tissue-specific or developmentalstage-specific expression of any of the 5'-UTR-specific transcriptsin other tissues analyzed (thymus, spleen, testis, ovary, muscle,liver, and different brain regions).

Next, we investigated the expression pattern of rREST1 mRNA. RPA analysis revealed that uniformly low levels of rREST1 mRNAare present in all tissues that were analyzed. In adult brainrREST1 mRNA constitutes ~10% and in non-neuronal tissues ~5% ofthe total rREST mRNAs (Fig. 5A). Because rREST1 mRNA is of relativelylow abundance, RT-PCR was performed to examine which of the 5'-UTRsare included in rREST1 mRNAs. RT-PCR analyses of RNA from embryonicor adult brain and thymus and sequence analyses of the PCR productsshowed that rREST1 transcripts with all of the different 5'-UTRsare present in the tissues that were analyzed. Using RT-PCR, weanalyzed brain and thymus RNA with the rREST1 3'-UTR-specificprimer in combination with primers specific for zinc fingers 5,6, 8, and 9 (see Materials and Methods and Fig. 8A) to ascertainthat rREST1 cDNA was not a partially spliced transcript. Primerpairs that would amplify the corresponding fragments of full-lengthrREST mRNA were used as controls. No amplification products weredetected with rREST1-specific primer combinations.

However, two distinct PCR products differing in size by ~30 bp were identified in the cDNA of brain while the regions fromzinc finger 2 to zinc finger 6 or from zinc finger 2 to zinc finger8 (p2^s-p6^as and p2^s-p8^as; see Materials and Methods) were amplified. Sequence analysisrevealed that some of the PCR clones represented unique rRESTtranscripts with either partial loss of the coding sequences (rREST3)or short insertions of novel sequences (rREST2, +4 bp; rREST4,+16 bp; and rREST5, +28 bp) in the region encoding the spacerbetween zinc finger motifs 5 and 6 (Fig. 8B). All three differentinsertions as well as the novel deletion led to translationalframe shifts that predict truncated forms of rREST protein withfive zinc finger motifs (Fig. 8B,C). The expression levels ofrREST splice variants encoding truncated proteins were analyzedby RPA, using the probe spanning the spacer region between zincfingers 5 and 6 (riboprobe 5; see Materials and Methods and Fig.1B). A fully protected fragment (360 bp) corresponding to thefull-length rREST mRNA was seen in all tissues that were analyzed,whereas a shorter (346 bp) fragment was detected specificallyin neural tissues (various brain regions and during brain development;Fig. 5C). The shorter protected fragment represented a mixed populationof rREST2, rREST3, rREST4, and rREST5 transcripts that divergefrom the full-length rREST mRNA in a defined residue after zincfinger 5 motif. RPA analysis of rREST4 mRNA revealed its neural-specificexpression pattern, with the highest levels in embryonic brain(~1% of total rREST mRNA) and in the cultured cortical neurons(~30% of total rREST mRNA), whereas no expression was detectedin non-neuronal tissues and in the cultured astrocytes (Fig. 5C).Because of the detection limit of RPA method, we were not ableto detect rREST2, rREST3, and rREST5 mRNAs, indicative of theirextremely low abundance. RT-PCR analyses of RNA from several tissuesconfirmed the neural-specific expression of rREST4 and rREST5mRNAs and identified the presence of rREST2 and rREST3 mRNAs inall analyzed tissues of both neuronal and non-neuronal origin(Fig. 6A). By means of RT-PCR we also established that these low-abundantrREST transcripts had no bias for any particular 5'-UTR sequence(Fig. 6B).

View larger version (42K):
[in this window]
[in a new window]
Figure 6. RT-PCR analysis of the expression of rREST transcripts encoding truncated rREST protein isoforms with five zinc finger motifs.Shown are ethidium bromide stains of 2% agarose gels. Poly(A⁺) RNA (500 ng) was reverse-transcribed; 35 cycles of PCR amplificationwere performed in A, and 45 cycles were performed in B. Each lanecontains one-fifth of the RT-PCR reaction. A, Expression of rREST2,rREST3, rREST4, and rREST5 mRNAs during rat brain developmentand in non-neuronal tissues. Note that rREST2 and rREST3 mRNAare expressed during brain development and in non-neuronal tissues,whereas expression of rREST4 and rREST5 mRNA is detected exclusivelyin the brain at different stages of development. RT-PCR analysiswas performed by using primer sets specific to rREST2 mRNA (p2^s-pR2^as), rREST3 mRNA (p2^s-pR3^as), rREST4 mRNA (p2^s-pR4^as), and rREST5 mRNA (p2^s-pR5^as) (see also Materials and Methods and Fig. 8A). B, Expressionof rREST2, rREST3, rREST4, and rREST5 mRNAs with different 5'-UTRsof type A (lanes 1-3), type B (lanes 4-6), and type C (lanes 7-9)in the brain (lanes 1, 4, 7) and thymus (lanes 2, 5, 8). Notethat all of these truncated rREST transcripts exhibit no biasfor any particular 5'-UTR sequence. RT-PCR analyses that wereperformed are not quantitative and show only the presence or absenceof the rREST transcripts analyzed. Primer combinations that wereused include the following (see also Materials and Methods andFig. 8A): lanes 1-3, pA^s in combination with pR2^as, pR3^as, pR4^as, or pR5^as; lanes 4-6, pB^s in combination with pR2^as, pR3^as, pR4^as, or pR5^as; lanes 7-9, pC^s in combination with pR2^as, pR3^as, pR4^as, or pR5^as. $-$ RT in A and lanes 3, 6, and 9 in B are negative controls forwhich no cDNA was added to the PCR reaction.

Our data show that the expression levels of different rREST transcripts in the brain are in the following rank of abundance:rREST (90% of all rREST transcripts) > rREST1 (~10%) > rREST4(1%) > rREST2 = rREST3 = rREST5 (each < 0.1%). In the non-neuronaltissues, approximate levels of rREST transcripts are rREST (95%)> rREST1 (~5%) > rREST2 = rREST3 (each $<=$ 0.1%). These relativelevels of abundance, together with the in situ hybridization data,suggest that the major transcript expressed in neurons encodesrREST protein with nine zinc fingers.

Structure of the rat REST/NRSF/XBR gene

The possibility that different transcripts could be generated by alternative splicing motivated us to characterize the rRESTgene structure. The human REST/NRSF/XBR mRNA has been shown previouslyto be encoded by a single-copy gene (Scholl et al., 1996). Southernblot analysis of rat genomic DNA at high- and low-stringency conditionswith different probes showed that rREST is encoded by a single-copygene (Fig. 7). Because all the signals detected at low-stringencywashing conditions also were seen after high-stringency washes,we concluded that the REST/NRSF/XBR has no close homologs in therat genome. Alternatively, if rREST homologs exist, they wouldshare low relatedness within the zinc finger region, which, however,remained below the detection limit of our Southern hybridizationmethod.

View larger version (60K):
[in this window]
[in a new window]
Figure 7. Southern blot analysis of rREST gene. Rat genomic DNA was digested with the indicated restriction enzymes. Two identical filterswere hybridized with probes corresponding to different regionsof rREST cDNA. Left, Hybridization with the 460 bp PvuII/AvaIIrREST cDNA fragment (riboprobe 4; see Materials and Methods) spanningthe region encoding part of the N terminus up to the zinc finger2 motif. Right, Hybridization with the 360 bp AvaII/DraI rRESTcDNA fragment (riboprobe 5; see Materials and Methods) coveringthe region from the zinc finger 2 motif up to the zinc finger6 motif. The detection of two genomic DNA fragments of differentsizes in both lanes of the right panel indicates that at leastone intron is present in the region encoding the N-terminal zincfinger cluster. The DNA molecular weight size markers (in kb)are indicated at left.

To characterize the structure of the rREST gene further, we applied long-distance PCR of rat genomic DNA, using primers specificfor different 5'-UTRs, the region of translation initiation, andindividual zinc finger motifs (see Materials and Methods and Fig.8A). Sequence comparison of the amplified genomic fragments withrREST cDNA revealed that rREST gene consists of at least six exonsand identified the splice site sequences of exon/intron boundaries(Table 2), which are all in agreement with the respective consensussequences (Csank et al., 1990). The results of the structuralanalysis of rREST gene are depicted in Figure 8 and summarizedas follows.

View larger version (33K):
[in this window]
[in a new window]
Figure 8. Structure of the rREST gene and alternative transcripts. A, The structural organization of rREST gene determined by PCR analysisof genomic DNA. Exons are shown as boxes, and introns are shownas lines. The numbers above the introns indicate their respectivesizes. Short black bars with primer-specific identification symbolsshown above or below the exons indicate the position of the senseor antisense primers used in PCR analyses. The putative extensionof exon IV is shown with the dashed stroke. The vertical graybars indicate zinc finger motifs. Exon numbers in bold Roman charactersfrom I to VI are shown below the respective exons; the neural-specificexon located between exons V and VI is indicated as N. The schematicrepresentation of rREST transcripts in relation to the gene isshown below the gene structure. Alternatively spliced rREST transcriptsare shown. 5'-UTRs of types A, B, and C are indicated as openboxes. Dashed lines and lines indicate the regions that are splicedout from the primary transcripts. Dashed lines also show the usageof alternative 5'-UTRs. 3'-UTRs are shown as open boxes with dashedstrokes. The ORF of each rREST transcript is indicated as a filledbox. B, Alternative splice sites for exons V, N, and VI. Exonsequences are given in capital letters and are boxed. Alternativelyspliced sequences are indicated as striped boxes. Lines indicatethe regions that are spliced out of the primary transcript. rREST4and rREST5 transcripts are the products of neuron-specific splicingwith the insertion of either partial or entire exon N, shown asstriped boxes between exons V and VI. C, Partial alignment ofrREST cDNAs in the region that follows zinc finger 4 (rREST1)or zinc finger 5 motif (rREST2-5), where the introduced terminationcodons lead to altered ORFs. The amino acid sequences of the predictedproteins are shown. The termination codons are indicated by anasterisk.


View this table:
[in this window]
[in a new window]
Table 2. Intron/exon boundary sequences of the rat rREST gene

All of the different 5'-UTRs are encoded by separate exons (exons I, II, and III, respectively) and predisposed to alternativesplicing (Table 2; Fig. 8A). We could not determine the sizeof the intron separating exon I encoding the type A 5'-UTR fromexon IV encoding the beginning of the protein coding region, mostlikely attributable to its large size, because we could amplifyfragments up to 15 kb by using the same genomic DNA as a templatewith other primer combinations. In contrast, the introns separatingexon II (5'-UTR-B) from exon III and exon III (5'-UTR-C) fromexon IV are relatively short, 1.5 and 1.2kb of length (Fig. 8A),respectively.

Exon IV (905 bp) is coding the region from the translation initiation codon up to the end of zinc finger 4 motif and is separatedby a 7.5 kb intron from exon V. Exon V is 84 bp long and encodesthe spacer between zinc fingers 4 and 5 and the entire zinc finger5 motif. rREST1-specific 3'-UTR is encoded by intron IV (Fig.8B), suggesting a mechanism of splicing in which intron IV isretained in the moiety of mature rREST1 mRNA. Intron retentiontype splicing is suggested to be a rarely detected splicing phenomenon(Nakai and Sakamoto, 1994). Although the molecular basis for therREST1 pre-mRNA processing still remains obscure, it results inthe translational frame shift and predicts a rREST isoform (rREST1^trunc), which is one-third of the size of rREST protein.

The intron separating exon V from exon VI is ~6 kb long. Exon VI contains the region of rREST encoding zinc fingers 6-9 (Fig.8A). Alignment of different rREST cDNAs with the sequence of theintron separating exon V from exon VI revealed the following (Table2; Fig. 8): (1) rREST2 containing a 4 bp (gttg) insertion originatesfrom the usage of a cryptic splice donor site located immediatelydownstream from the authentic one, (2) rREST3 with partial lossof coding sequences (corresponding to amino acids 327-329) resultsfrom the usage of a cryptic splice acceptor site located withinexon V, and (3) rRESTR4 and rREST5 are generated by alternativesplicing of a neuron-specific (N) exon that is located 5.2 kbdownstream of exon V and 0.8 kb upstream of exon VI. The varyinglength of the inserted exon N in the processed transcripts reflectsthe use of two different splice donor sites. All of these secondarysplicing patterns lead to translational frame shifts and predicttruncated isoforms of rREST protein with five zinc finger motifs.

Slow onset and prolonged activation of REST/NRSF/XBR gene after kainate-induced seizures

Neuronal activity has been shown to alter the expression of various genes in adult neurons. These alterations are thoughtto be involved in long-lasting or adaptive changes leading tosynaptic reorganization (Ben-Ari and Represa, 1990) or persistinghyperexcitability (Meier et al., 1992) associated with LTP orepilepsy, accordingly. Because in certain experimental seizuremodels the transcription of some of the rREST target genes hasbeen shown to be modified, we studied the effect of KA-inducedseizures on the expression of rREST transcripts in the adult ratbrain (Fig. 9). RPA analyses revealed a similar pattern of inductionof rREST1, rREST4, and rREST mRNAs in the hippocampus at 4 hrafter injection of KA; the levels remained elevated up to 24 hrafter treatment, the last time point analyzed (Fig. 9A). Usingin situ hybridization, we observed a pronounced increase in rRESTmRNA levels in the hippocampal formation in the granular neuronsof dentate gyrus at 4 hr after the injection of KA (Fig. 9B).At 24 hr, rREST mRNA levels in the dentate gyrus had decreased,whereas a significant increase in rREST mRNA levels was observedin the pyramidal layers CA1-CA4. Notably increased levels of rRESTmRNA expression were seen also in the external and internal layersof cerebral cortex (Fig. 9B) and piriform cortex.

View larger version (69K):
[in this window]
[in a new window]
Figure 9. Expression of rREST mRNA in the hippocampus after kainic acid treatment. A, RPA of rREST1, rREST4, and rREST mRNA expressionin the hippocampus at 2, 4, and 24 hr after KA-induced seizures.The amount of RNA used in RPA was 20 µg for rREST1 transcripts(riboprobe 6; see Materials and Methods and Fig. 1B) and 40 µgfor rREST4 transcripts (riboprobe 9; see Materials and Methodsand Fig. 1B). Total RNA was isolated from the hippocampus of saline-or KA-treated animals. Protected fragments corresponding to rREST1,rREST4, rREST, and GAPDH mRNA are indicated. Saline treatmentwas performed for 2, 4, and 24 hr; no changes were detected inthe expression levels of any of the rREST transcripts. B, Dark-fieldautoradiographs showing rREST mRNA-specific labeling in the adultrat brain at 4 and 24 hr after KA-induced seizures. Coronal sectionswere prepared at the level of dorsal hippocampus and hybridizedwith the rREST-specific cRNA probes (riboprobes 4 and 11; seeMaterials and Methods and Fig. 1B). contr., Endogenous levelsof corresponding rREST transcripts in hippocampus; saline, levelsof rREST1, rREST4, and rREST transcripts 4 hr after saline treatment;KA, kainic acid; tRNA, yeast tRNA as a negative control; SENSE,section hybridized with the [ $alpha$ -³⁵S]-labeled sense riboprobe; CP, choroid plexus; dg, dentate gyrusof the hippocampus; CTX, cerebral cortex; CA1, CA3, CA4, pyramidallayers CA1, CA3, and CA4 of the hippocampus.

REST/NRSF/XBR protein isoforms convey transcriptional repression

We generated a series of C-terminal deletion mutants that correspond to the predicted truncated forms of rREST protein tostudy their functional role, using transient expression assays.Expression plasmids of various rREST deletion mutants (see Materialsand Methods) were cotransfected, along with the thymidine kinase(TK) promoter-based reporter construct (pNRSE^BDNFCAT), in mouse neuroblastoma Neuro-2A and rat glioma C6 cellsand were analyzed with chloramphenicol acetyltransferase (CAT)assays. pNRSE^BDNFCAT contains a palindromic NRSE originating from the promoterII region of the rat BDNF gene (NRSE^bdnf) (Timmusk et al., 1993) linked to the TK promoter.

First, we determined the levels of REST/NRSF/XBR mRNA in Neuro-2A and C6 cells. RPA analysis revealed that rREST full-lengthmRNA is the major transcript (~200 molecules per cell) in C6 cells,whereas the major transcript in Neuro-2A cells is a splice variantthat corresponds to the neural-specific rREST4 mRNA (~50 moleculesper cell). In Neuro-2A cells the REST/NRSF/XBR full-length mRNAwas not detectable, even by means of RT-PCR method.

In Neuro-2A cells, increasing amounts of the plasmid encoding rREST protein led to the concentration-dependent repressionof the pNRSE^BDNFCAT activity (Fig. 10A). Both deletion mutants of rREST correspondingto the natural truncated isoforms with five (rREST2-5^trunc) or four zinc finger motifs (rREST1^trunc) acted also as transcriptional repressors in Neuro-2A cells (Fig.10B). Expression of rREST2-5^trunc resulted in relatively weak (3.2-fold) repression, whereas expressionof rREST1^trunc resulted in strong repression (6.7-fold) of the pNRSE^BDNFCAT promoter activity in Neuro-2A cells. Next, we tested the transcriptionalactivities of rREST deletion mutants in C6 cells in which theendogenous levels of rREST full-length mRNA are high. In C6 cells,overexpression of rREST and rREST2-5^trunc resulted in relatively weak (3.7- and 2.7-fold, respectively)repression, as compared with overexpression of rREST1^trunc, which resulted in strong repression (6.5-fold) of the reportergene activity (Fig. 10B). To exclude the possibility that silencingactivity resides in the pBLtkCAT vector backbone, we also performedtransfection assays, using pBLtkCAT as a reporter gene. Our datarevealed that repression mediated by rREST and its deletion mutantsis attributable to NRSE in pNRSE^BDNFCAT construct, because we could not detect any changes in TK promoteractivity in response to the overexpression of rREST or its deletionmutants (data not shown).

View larger version (49K):
[in this window]
[in a new window]
Figure 10. Effects of rREST and rREST-truncated isoforms on pNRSE^BDNFCAT promoter activity in Neuro-2A and C6 cells. A, rREST represses pNRSE^BDNFCAT activity in a concentration-dependent manner. Transient transfectionassays were performed in Neuro-2A cells, using 2 µg of pNRSE^BDNFCAT and various amounts of plasmid encoding rREST protein, asindicated. Acetylated (Cm-3-Ac) and nonacetylated (Cm) forms ofchloramphenicol are indicated on the left. CAT activity of pNRSE^BDNFCAT in the presence of pcDNA3 alone was assigned a level of 100%activity. Repression (fold) is calculated as 100% $div$ CAT activityat a given plasmid concentration. Shown are the calculated valuesof one experiment; however, similar results were obtained in fourindependent experiments. B, Effects of rREST and rREST-truncatedisoforms on pNRSE^BDNFCAT activity. Shown is a schematic representation of rREST proteinand the rREST-truncated isoforms; the last amino acid is indicatedon the right, and the designation of the construct is shown onthe left. Black boxes represent zinc fingers. The pNRSE^BDNFCAT reporter plasmid was cotransfected with 15 µg of parentalpcDNA3 or with 15 µg of recombinant expression vectors of rRESTor rREST-truncated isoforms. In the table at right, the valuesdenoting repression were calculated as described in A of thisfigure and represent averages of at least four independent experimentsperformed in triplicate. SEM is shown. C, Gel retardation assaysshowing the DNA binding activity of rREST isoforms (rREST1^trunc and rREST2-5^trunc), the deletion mutant with seven zinc fingers (rREST402D), andrREST protein to the wild-type palindromic NRSE^bdnf sequence derived from the promoter II region of BDNF gene. Theradiolabeled DNA fragment containing NRSE^bdnf was incubated in the binding buffer with the in vitro translatedprotein products in the presence of the nonspecific competitoror 100-fold excess of the specific competitors, the unlabeledoligonucleotides corresponding to the upper (lane +11) or lower(lane +21) half site of NRSE^bdnf. The DNA-protein complexes were resolved by native 5% PAGE electrophoresis.D, In vitro translation analyses of equimolar amounts of differentrREST expression plasmids. [³⁵S]methionine-labeled protein samples were analyzed by 12.5% SDS-PAGEelectrophoresis. Molecular weight size standard markers are shownon the left.

Because both truncated isoforms of rREST caused effects of similar magnitude in different cellular contexts, it suggests thattruncated rREST isoforms convey repression independent of thetranscriptional activities of endogenous rREST proteins. Duringthe revision of this manuscript Tapia-Ramirez et al. (1997) identifiedthe presence of two distinct repressor domains located at oppositeends of the REST/NRSF/XBR molecule, using the GAL4 expressionsystem. Because the N terminus of REST/NRSF/XBR is highly conservedbetween rat and human (Fig. 1A), the repressor activity of rREST-truncatedisoforms apparently originates from the N terminus.

We performed gel retardation assays to investigate whether rREST-truncated isoforms with four or five zinc fingers (rREST1^trunc and rREST2-5^trunc) are capable of binding to NRSE^bdnf in vitro. As shown in Figure 10C, rREST with the intact nine zincfinger DNA binding domain and rREST deletion mutant with sevenzinc fingers (rREST402D) could form sequence-specific retardedcomplexes with the upper half site of the palindromic NRSE^bdnf motif. However, by means of our assay we were not able to detectany DNA-protein complexes in the samples containing rREST2-5^trunc or rREST1^trunc. Equimolar amounts of expression plasmids yielded similar amountsof proteins, as shown by in vitro translation analysis (Fig. 10D),indicating that the absence of shifted complexes was not attributableto the differences in the protein expression levels.

Taken together, these data suggest the following: (1) the truncated forms of rREST protein individually may affect gene transcriptionwithout interfering with rREST-mediated effects, and (2) lossof the region between zinc finger motifs 5 and 9 leads to theloss of binding of rREST protein isoforms to the NRSE of rat BDNFgene in vitro.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The main conclusions of the present study are the following: (1) alternative splicing is used in the regulation of rat REST/NRSF/XBR(rREST) gene to generate multiple transcripts with differentialexpression profiles; (2) different rREST splice variants are expressedin mature neurons of adult brain; (3) rREST mRNA levels are inducedin the hippocampal and cortical neurons by neuronal activity;(4) alternatively spliced rREST transcripts encode protein isoformsthat differ in their DNA binding specificity, and all mediaterepression of transcription.

We show that rREST shares overall 70% amino acid identity with the human REST/NRSF/XBR protein, exhibiting poor homology inthe region separating the N- and C-terminal zinc finger clusters(the amino acid identity is ~50%). Partial analysis of the structuralorganization of the gene reveals the presence of three intronsin the region encoding the N-terminal zinc finger cluster of rRESTprotein. Modular structure of rREST gene with separate exons encodingfunctionally defined domains reflects the divergent evolutionaryorigin of these distinct structural units. On the other hand,modular structure provides the basis for regulation of rREST geneexpression by alternative splicing.

Our data reveal multiple splicing patterns of rREST pre-mRNA. Most striking is the finding that all of the different rRESTsplice variants are expressed in adult brain neurons. Anotherinteresting finding is that the splicing pattern that involvesthe insertion of a short exon (exon N) is only characteristicto neurons and results in two neuron-specific splice variants,rREST4 and rREST5. rREST4 and rREST5 mRNAs encode truncated rRESTprotein isoforms with five zinc fingers as a result of the frameshift introduced by exon N. Neuron-specific splicing of shortexons has been described, for example, in c-src (Levy et al.,1987; Martinez et al., 1987), trkA (Barker et al., 1993), andnonmuscle myosin heavy chain-B (MHC-B) genes (Takahashi et al.,1992). The biological significance of neuron-specific splicingin rREST gene regulation currently remains unclear, because theexpression levels of exon N-containing rREST transcripts in adultrat brain are much lower than the levels of rREST transcriptsin which exon N is not included. All other forms of rREST pre-mRNAsplicing are common to structures of both neuronal and non-neuronalorigin. The dominant splicing pattern involves exon N skippingand results in rREST transcript with the longest ORF. Of all ofthe rREST transcripts expressed in the brain, 90% exhibit exonN skipping and encode rREST protein with the DNA binding domainof nine zinc fingers. Two secondary patterns of splicing may occursimultaneously with exon N skipping. These are caused by the activationof cryptic splice sites and result in splice variants (rREST2and rREST3) that encode truncated forms of rREST protein withthe DNA binding domain of five zinc fingers. rREST2 and rREST3show the lowest levels of expression of all of the rREST transcripts,both in neuronal and non-neuronal tissues. rREST1 mRNA, whichencodes a protein with the DNA binding domain of four zinc fingers,also is widely expressed in neuronal and non-neuronal structures.The molecular basis for this type of splicing is currently unclear;however, it appears to be conserved across species because a humanEST displays high sequence homology to the rREST1 cDNA.

Previous studies detected abundant expression of REST/NRSF/XBR mRNA in most of the non-neuronal tissues during developmentand also in undifferentiated neuronal progenitors, but not indifferentiated CNS neurons. These results suggested that REST/NRSF/XBRis a transcription factor that controls neurogenesis (Chong etal., 1995; Schoenherr and Anderson, 1995a). Here, we propose that,in addition to its role during neurogenesis, REST/NRSF/XBR alsois involved in maintaining neuronal identity by quantitativelymodulating the expression level of its target genes. We provideseveral pieces of evidence to support this hypothesis.

First, we demonstrate that rREST mRNA is differentially expressed in the mature neurons of adult brain. The highest levelsof rREST mRNA were detected in the neurons of hippocampus andthe nuclei of pons/medulla and midbrain. Previous studies haveshown that neuronal genes that contain NRSE-like sequences (Schoenherret al., 1996) may convey NRSF/REST/XBR-mediated repression (Kraneret al., 1992; Mori et al., 1992; Pathak et al., 1994; Thiel etal., 1994; Lönnerberg et al., 1996; Mieda et al., 1996; Woodet al., 1996). Analyses of the data available in the literatureabout the expression profiles of REST/NRSF/XBR target genes revealedthat expression of some of these genes (M4 muscarinic receptor,NMDAR1, and GABA-A receptor) is limited to the brain regions inwhich rREST mRNA is not expressed or expressed at low levels.For example, M4 muscarinic receptor mRNA is highly expressed incaudate putamen (Vilaro et al., 1991), where rREST mRNA is notdetected. On the other hand, a majority of REST/NRSF/XBR targetgenes are expressed in most regions of adult brain. The high levelof expression of these target genes is found mostly in the regionsthat exhibit low levels of rREST mRNA. The expression patternof rREST mRNA shows an inverse correlation with the expressionof NaCh II (Brysch et al., 1991), SCG10 (Himi et al., 1994), calbindinI (Abe et al., 1992), synaptotagmin IV (Berto