The Human ARF Cell Cycle Regulatory Gene Promoter Is a CpG Island Which Can Be Silenced by DNA Methylation and Down-Regulated by Wild-Type p53

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Molecular and Cellular Biology, November 1998, p. 6457-6473, Vol. 18, No. 11
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

The Human ARF Cell Cycle Regulatory Gene Promoter Is a CpG Island Which Can Be Silenced by DNA Methylation and Down-Regulated by Wild-Type p53

Keith D. Robertson and Peter A. Jones^*

Norris Comprehensive Cancer Center, The University of Southern California, Los Angeles, California 90033

Received 21 April 1998/Returned for modification 24 May 1998/Accepted 6 August 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

The INK4a/ARF locus encodes two proteins involved in tumor suppression in a manner virtually unique in mammalian cells. Distinctfirst exons, driven from separate promoters, splice onto a commonexon 2 and 3 but utilize different reading frames to produce twocompletely distinct proteins, both of which play roles in cellcycle control. INK4a, a critical element of the retinoblastomagene pathway, binds to and inhibits the activities of CDK4 andCDK6, while ARF, a critical element of the p53 pathway, increasesthe level of functional p53 via interaction with MDM2. Here weclone and characterize the promoter of the human ARF gene andshow that it is a CpG island characteristic of a housekeepinggene which contains numerous Sp1 sites. Both ARF and INK4a arecoordinately expressed in cells except when their promoter regionsbecome de novo methylated. In one of these situations, ARF transcriptioncould be reactivated by treatment with the DNA methylation inhibitor5-aza-2'-deoxycytidine, and the reactivation kinetics of ARF andINK4a were found to differ slightly in a cell line in which bothgenes were silenced by methylation. The ARF promoter was alsofound to be highly responsive to E2F1 expression, in keeping withprevious results at the RNA level. Lastly, transcription fromthe ARF promoter was down-regulated by wild-type p53 expression,and the magnitude of the effect correlated with the status ofthe endogenous p53 gene. This finding points to the existenceof an autoregulatory feedback loop between p53, MDM2, and ARF,aimed at keeping p53 levels in check.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The INK4a/ARF (alternative reading frame) cell cycle regulatory locus has proven to be a unique and interesting experimentalsystem. The INK4a (p16 INK4a, MTS1, CDKN2, p16 $alpha$ ) gene was implicatedas a tumor suppressor gene by its frequent mutation, deletion,or promoter hypermethylation in a variety of human tumors (14,39; reviewed in reference 64). The role of the INK4a locusbecame more complicated with the finding of a second gene, ARF,which shares a portion of the INK4a coding region and has a uniquefirst exon (termed exon 1 $beta$ ) originating approximately 20 kb centromericto INK4a exon 1 (now termed exon 1 $alpha$ ) (reviewed in references 31,36, and 68). This exon, under the control of its own promoter,splices onto exon 2 of INK4a in an alternative reading frame,allowing for the production of two totally unrelated proteins,both of which are cell cycle regulators and tumor suppressorsin mouse models (27, 33, 52, 61). The critical importanceof this locus may lie in the involvement of its two gene productsin two of the most important cell cycle regulatory pathways: ARFin the p53 pathway and INK4a in the retinoblastoma gene product(pRb) pathway (reviewed in references 16 and 27).

Of the four known members of the INK4 family (p15 INK4b, p16 INK4a, p18 INK4c, and p19 INK4d), only INK4a has a firmly establishedrole in human tumorigenesis (23, 26). In addition to INK4amutations being associated with familial melanoma, mutation ordeletion of INK4a occurs with a frequency ranging from approximately30% in esophageal tumors to nearly 100% in pancreatic and non-small-celllung carcinomas (4; reviewed in references 17, 57, and59). The INK4 proteins can block cyclin D-dependent kinase (cdk)activities by preventing their association with the D-type cyclins,causing cells to arrest in G₁ (60; reviewed in reference 64).Arrest is mediated primarily through hypophosphorylation of pRb,a substrate of the cyclin D-cdk complex. pRb binds to and inhibitsa subset of transcriptional regulatory proteins termed the E2Fs,which then act as repressors of E2F target genes. Phosphorylationof pRb in these complexes allows the E2F proteins to transactivatetheir target genes, and their products then promote cell cycleprogression (reviewed in reference 64).

Another mechanism of INK4a inactivation that has been observed in cases in which no deletion or mutation could be found ispromoter region hypermethylation. The promoter of INK4a resideswithin a CpG island, and abnormal, tumor-associated hypermethylationhas been observed in many tumor types and found to result in silencingof the gene (14, 39). CpG islands are regions rich in theCpG dinucleotide which are often associated with genes and arenormally kept unmethylated in cells by an unknown mechanism butwhich may involve binding of the Sp1 transcription factor (35).

The newer member of the INK4a locus, ARF (murine p19 ARF and human p14 ARF [63, 65] and p16 $beta$ [33]), is predicted toencode a basic polypeptide with no homology to known proteinsand which shows approximately 50% identity between mouse and humanproteins (compared to 65% for INK4a). ARF is ubiquitously expressedand is elevated in cells lacking functional p53. ARF does notbind to cdks or inhibit the activities of cyclin-cdk complexes;however, overexpression of ARF results in cell cycle arrest inboth G₁ and G₂ (52). Mutations within exon 1 $beta$ have not beenreported; however, mutations within the shared exon 2 region,which inactivate INK4a, also have the potential to affect ARF,but no definitive mutations have yet been found in ARF that donot also disrupt INK4a (11, 51, 71). Large deletions ofthis region of chromosome 9p that remove INK4a would also likelyknock out ARF. The role of mutations in exon 2 of ARF is questionablein any case, since the cell cycle inhibitory functions of ARFare encoded entirely by sequences within the unique exon 1 $beta$ (51).The role of ARF in tumorigenesis was firmly established, at leastin mice, by recent work involving a targeted disruption of exon1 $beta$ . ARF-null mice developed lymphomas and sarcomas at an earlyage, a phenotype indistinguishable from that of a previous INK4aexon 2 knockout which effectively disrupted both INK4a and ARF(61). Furthermore, cell cycle arrest mediated by ARF was abolishedin cells lacking functional p53, indicating that ARF may act upstreamof p53 (reviewed in references 16, 27, and 48).

Recent work has shown that the role of ARF in the p53 pathway is to bind to MDM2 (48, 78). MDM2, a proto-oncogene itself,binds to p53 and targets it for degradation in the ubiquitin pathway,resulting in abrogation of its antiproliferative and apoptosis-promotingeffects (19, 30, 32, 42). MDM2 lso masks the p53 transcriptionalactivation domain (42, 43). In one study, ARF was shown tobind to and induce the degradation of the MDM2 proto-oncogene,resulting in a stabilization of p53 (78). In a second study,ARF was shown to suppress oncogenic transformation in a p53-dependentmanner, block MDM2's ability to mask the transcriptional activatingfunction of p53, and be necessary for the efficient executionof the p53-dependent apoptotic response (48). Regulation ofcell division and apoptosis by p53 is thought to be due to theability of p53 to modulate transcription of genes involved incontrolling both processes. p53, by virtue of its interactionwith many cellular proteins, has been shown to act as a sequence-specificDNA binding protein and transcriptional activator (8, 46)and also repress transcription from promoters which do not containp53 binding sites (6, 13, 34, 38, 58, 69) throughsequestration of the TATA binding protein (TBP) and inhibitionof transcriptional initiation (62).

The focus of this work was to gain a better understanding of the factors involved in regulating the INK4a/ARF locus. Specifically,we cloned and sequenced the promoter region of the human ARF geneand found that it possesses many of the features of a housekeepinggene. Gene expression studies indicated that ARF is ubiquitouslyexpressed in cell lines, with only two notable exceptions. Inthese two cases, promoter region hypermethylation was demonstratedby Southern blotting and ARF expression could be reactivated aftertreatment with the methylation inhibitor 5-aza-2'-deoxycytidine(5-aza-CdR). Promoter deletion analysis revealed the locationof potentially important regulatory regions, including numerousSp1 sites. Potential E2F binding sites were also detected, andthe ARF promoter was found to be highly responsive to E2F1 ashas been observed previously at the RNA level (9). Transfectionstudies with ARF and INK4a reporter constructs indicated thatthe transcription factors necessary for promoter activity wereubiquitously expressed and that the activities of the endogenousgenes were related to their methylation status. Lastly, studiescomparing the effects of wild-type p53 overexpression on ARF andINK4a promoter constructs indicated that transcription from theARF promoter could be potently repressed, in keeping with previousobservations at the protein level that ARF levels are elevatedin cells lacking functional p53. Thus, we propose the existenceof an autoregulatory feedback loop involving p53, MDM2, and ARFwhich functions to keep p53 levels tightly controlled in normalcells.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cell lines, tissue culture, and drug treatments. The colon cancer-derived cell lines HCT116, HCT15, SW48, LoVo, SW837, and HT-29 were maintained in McCoy's 5-a medium. Thebladder cancer lines 5637 and J82 and the cervical cancer lineC-33A were maintained in minimal essential medium supplementedwith sodium pyruvate and nonessential amino acids (Life Technologies).The lymphoid lines Raji, CA46, and HL-60 were maintained in RPMI1640. The hepatocellular carcinoma line Hep 3B and the bladdercell line T24 were maintained in Dulbecco modified Eagle medium,and the pancreatic line CFPac-1 was maintained in Iscove modifiedDulbecco medium. All media were supplemented with 10% fetal bovineserum (20% for the HL-60 line). All cell lines were purchasedfrom the American Type Culture Collection. For 5-aza-CdR (Sigma)treatments, cells were diluted to 3.0 × 10⁵/ml and allowed to grow overnight; then freshly prepared 5-aza-CdRwas added to a final concentration of 1.0 µM, and the cells wereallowed to grow for the times indicated. For DNA damage transfectionexperiments, camptothecin (CMT; Sigma) was used at a final concentrationof 5 µM in dimethyl sulfoxide (DMSO) and cytosine arabinoside(Ara-C; Oncogene Science) was used at a final concentration of50 µM in water. DMSO was also added to Ara-C cultures at the sameconcentration as that for the CMT treatments to control for nonspecificsolvent effects on cells.

Reverse transcription (RT)-PCR analysis of ARF and INK4a expression. Total RNA (2.5 µg) was isolated with Trizol (Life Technologies) and reverse transcribed by using gene-specific 3' primers,deoxynucleoside triphosphates (Boehringer Mannheim), and SuperscriptII reverse transcriptase (Life Technologies) in a 20-µl volume.The primers used were specific for INK4a and ARF (common antisense5'-TTC CCG AGG TTT CTC AGA G-3') and for PCNA (proliferating cellnuclear antigen) (antisense 5'-GCT AGG ATC CTA AGA TCC TTC TTCATC CTC GAT C-3'). cDNA was amplified by PCR with 5' primers specificfor ARF, INK4a, and PCNA with the same antisense primer used forcreation of cDNA. PCR was performed in a 50-µl volume as follows:for ARF and INK4a, 94°C for 2 min, followed by 35 cycles at 94°Cfor 30 s, 58°C for 1 min, and 72°C for 1 min; for PCNA, 94°C for2 min, followed by 35 cycles at 94°C for 30 s, 60°C for 1 min,and 72°C for 1 min. 5' primers were 5'-CAT GGT GCG CAG GTT CTTG-3' for ARF, 5'-AAC GCA CCG AAT AGT TAC G-3' for INK4a, and 5'-GATCGG ATC CGT ATG TTC GAG GCG CGC CTG GTC-3' for PCNA. PCR productswere resolved on 1.2% agarose gels, transferred to nylon membranes(NEN), and probed as described previously (56) with the followingend-labeled primers: for ARF, 5'-TAC TGA GGA GCC AGC GTC TAG-3'(exon 1 $beta$ ); for INK4a, 5-TAC TGA GGA GCC AGC GTC TAG-3' (exon 1 $alpha$ );and for PCNA, 5-CTA GCG CCA AGG TAT CCG CG-3'. Quantitation wasperformed on a Molecular Dynamics PhosphorImager.

Cloning and sequencing of the human ARF promoter. A lambda genomic library (human placenta) was probed with an exon 1 $beta$ -specific probe according to instructions of the manufacturer(Stratagene). The probe was generated by PCR using the sense primer5'-GAT CGC ATG CTC CCA GTC TGC AGT TAA GG-3' and antisense primer5'-GAT CGT CGA CGT CTA AGT CGT TGT AAC CCG-3', based on the previouslypublished exon 1 $beta$ sequence (36), and cloned into the TA cloningvector (Invitrogen). PCR conditions were similar to those usedfor ARF/INK4a RT-PCR, with 10% DMSO added and 50 ng of human placentalDNA (Sigma) as the template. A single phage clone was isolated,the insert was characterized by restriction analysis, and an approximately8.5-kb SacI fragment was subcloned into the SacI site of pBluescriptII (Stratagene) to create pKR19. The SacI site at the 3' end ofthis fragment corresponded to the SacI site at +49 of the previouslypublished sequence. All numbering is relative to the previouslypublished transcription start site (36). This fragment was furthersubcloned, and the region from +49 to $-$ 5650 was sequenced. A detaileddescription of subcloning procedures and sequencing primers willbe furnished upon request; note that only a portion of the regionsequenced is shown in Fig. 2B. All DNA sequencing was performedat the USC DNA Sequencing Core Facility.

Plasmid constructs. All ARF CAT promoter constructs were derived from pKR19. Initially, the SphI ( $-$ 5502)-PstI ( $-$ 18) fragment from pKR19 was clonedinto these same sites of pCAT-Basic (Promega) to create pKR21-3.This construct lacked the native transcription start site, whichwas added back by digesting pKR21-3 with SalI and cloning theSalI fragment derived from pKR19 (containing the ARF sequencesfrom $-$ 735 to +49 and a SalI site derived from pBluescript II)into this same site and screening for proper orientation to createp( $-$ 5502)19ARF. All subsequent deletion constructs had the same3' end at the +49 SacI site. 5'-end deletions were then made bydigesting p( $-$ 5502)19ARF with HindIII (within the pCAT-Basic vectorpolylinker) and a second enzyme within the ARF sequence, bluntingthe ends with T4 DNA polymerase (Boehringer Mannheim), and recircularizingwith T4 DNA ligase (Boehringer Mannheim). The second restrictionenzyme sites and the deletion constructs created were as follows:BstXI for p( $-$ 4690)19ARF, KpnI for p( $-$ 3407)19ARF, SpeI for p( $-$ 2465)19ARF,Eco47III for p( $-$ 925)19ARF, SmaI for p( $-$ 776)19ARF, SacII for p( $-$ 331)19ARF,BglII for p( $-$ 151)19ARF, and BssHII for p( $-$ 67)19ARF. p( $-$ 44)19ARFand p( $-$ 19)19ARF were created by PCR with p( $-$ 151)19ARF as the template(10 ng), a common 3' primer located within the vector sequence(5'-CAA CGG TGG TAT ATC CAG TG-3'), and 5' primer 5'-AGT CGG CATGCG CAG GGG GCG GTG CGT GGG-3' for the $-$ 44 construct or 5'-AGCTAG CAT GCT CTG CAG TTA AGG GGG CAG G-3' for the $-$ 19 construct.PCR conditions were the same as those used for ARF/INK4a RT-PCRanalysis except that Pfu DNA polymerase (Stratagene) was used.The PCR product was digested with SphI (incorporated into 5' primer)and SalI (derived from pCAT-Basic vector sequences) and clonedinto these same sites of pCAT-Basic. All sequences were confirmed.All INK4a promoter constructs were created by PCR with Pfu DNApolymerase and the previously described (15) INK4a promoter-containinglambda phage clone as the template. All constructs were namedrelative to the 5'-most transcription start site for INK4a, whichcorresponds to $-$ 306 relative to the translation start site andwhich contains all of the previously mapped transcription startsites (18). A common 3' primer was used for all constructs at+100 (5'-GCT AGT CGA CGG AGG AGG TGC TAT TAA CTC-3'), and 5' primerswere 5'-GAT CGC ATG CCA AAC ACG CCT TTG CTG GCA-3' for p( $-$ 118)16INK4a,5'-GAT CGC ATG CGG GGC TCT CAC AAC TAG GAA-3' for p( $-$ 293)16INK4a,5'-GAT CGC ATG CCC AGA CAG CCG TTT TAC ACG-3' for p( $-$ 474)16INK4a,5'-GAT CGC ATG CAG CAC TTT TTC TGG TCT AGG A-3' for p( $-$ 654)16INK4a,and 5'-GAT CAA GCT TGA ACT TTT ACC TCC TTG CGC-3' for p( $-$ 1729)16INK4a.The sequence of each construct was confirmed. Each PCR productwas digested with SphI [incorporated into the 5' primer; HindIIIwas used for p( $-$ 1729)16INK4a] and SalI (incorporated into the3' primer) and cloned into these same sites of pCAT-Basic. Thecontrol consensus p53 binding site chloramphenicol acetyltransferase(CAT) plasmid [2X(p53)BSCAT] was created by annealing complementaryoligonucleotides (top strand, 5'-GAT CTA GGC ATG CCT AGG CAT GCCTAA AGG CAT GCC TAG GCA TGC CTA-3') containing two copies of aconsensus p53 binding site (46). When annealed, BglII site overhangswere created and used to clone the oligonucleotide into the BglIIsite of pGH262 (provided by Gary Hayward, The Johns Hopkins University)to create 2X(p53)BSCAT. The p53 promoter-CAT plasmid (p53proCAT)was created by PCR as described for the INK4a reporter constructswith 5' primer 5'-ACT GAG CAT GCG GGA GAA AAC GTT AGG GTG TGG-3',3' primer 5'-GTG GCT CTA GAC TTT TGA GAA GCT C-3', and human placentalDNA as the template. The product was digested with SphI and XbaIand ligated into these same sites of pCAT-Basic to create p53proCAT,which contains the region from $-$ 96 to $-$ 534, relative to the translationstart site, of the human p53 promoter (73).

Transfection, CAT assay, and in vitro methylation. Cells were transfected with Lipofectamine as instructed by the manufacturer (Life Technologies). Briefly, 6 × 10⁵ cells were incubated in the presence of 2 µg of CAT plasmid and8 µl of Lipofectamine in the absence of serum for 7 h. Cell extractswere prepared 48 h later for CAT and $beta$ -galactosidase assays asdescribed previously (15, 56). Most CAT plasmid vectors werecotransfected with pSV40LacZ (15), and CAT activity was normalizedrelative to $beta$ -galactosidase activity to control for differencesin transfection efficiency. For the p53 dose-response transfections,2 µg of CAT plasmid was used along with a total of 2 µg of expressionvector. The amount of wild-type or mutant p53 expression vectorwas kept constant at 2 µg by addition of parental expression vectorcontaining no cDNA insert. Wild-type p53 (pC53-SN3), mutant p53(pC53-SCX3), and parental expression vector (pCMVNeoBam) werekindly provided by Bert Vogelstein (The Johns Hopkins University).For DNA damage transfections, cells were transfected identicallyexcept that drug was added with serum-containing medium 7 h aftertransfection, the cells were incubated overnight, and fresh mediumwas added the following morning. The total transfection time remainedthe same, 48 h. CAT activities were normalized to the proteinconcentration to account for small toxicity differences. Proteinconcentrations were determined with the Bio-Rad protein assayreagent according to the manufacturer's instructions. For E2F1response element mapping experiments, 2.0 µg of reporter plasmidwas cotransfected with 2.0 µg of E2F1 expression vector (providedby Joseph Nevins, Duke University) or empty parental expressionvector [pcDNA 3.1(+); Invitrogen]. In vitro methylation reactionswere carried out as described previously (55) with methylasespurchased from New England Biolabs. The completeness of the methylationreaction was confirmed by digestion of an aliquot of the reactionwith an appropriate methylation-sensitive restriction enzyme (HpaIIor HhaI). Quantitation of CAT activity was performed on a MolecularDynamics PhosphorImager.

Methylation analysis. Ten micrograms of genomic DNA was isolated from cell lines by standard procedures, digested with 100 U of each of the restrictionenzymes described in Results, resolved on a 1% agarose gel, transferredto a nylon membrane (NEN), and probed with ARF promoter-derivedfragments as described previously (25, 55). Double digestionswere performed sequentially, so that each restriction enzyme wasin the optimal incubation buffer with a precipitation step inbetween. All enzymes were purchased from New England Biolabs,and digestions were performed according to the manufacturer'sinstructions.

Nucleotide sequence accession number. The DNA sequence of the human ARF promoter has been deposited in GenBank under accession no. AF082338.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Analysis of ARF and INK4a expression patterns in cell lines and evidence for suppression by DNA methylation. We initially screened a panel of tumor cell lines derived from a variety of different tissues for both ARF and INK4a expressionby RT-PCR (Table 1 and Fig. 1A). Expression of ARF was observedin all tumor cell lines examined except the colon cancer celllines HCT15 and LoVo (Table 1; note that cell lines with knowndeletions of this region were excluded from this analysis). Expressionof INK4a was more restricted, and the data summarized in Table1 indicated that there were three expression patterns from theINK4a/ARF locus: (i) ARF⁺ INK4a⁺, (ii) ARF⁺ INK4a, and (iii) ARF INK4a. Interestingly we found no cell line in which ARF INK4a⁺ was the pattern. A large body of work has shown that the promotersof INK4a and p15 INK4b can become de novo methylated and silencedin tumor cells (14, 20, 39). It was therefore possible thatARF, which resides between these two genes, might be subject tosuch silencing.

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TABLE 1. Analysis of INK4a and ARF expression in cell lines by RT-PCR^a

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FIG. 1. (A) RT-PCR analysis of ARF (top) and p16 INK4a (bottom) expression patterns in the HCT15 cell line after treatment with 1.0 µM 5-aza-CdR for the times indicated. Also shown is a single time point (72 h) for the SW48, HCT116, and Raji cell lines. Hep 3B RNA was used as the positive (+) control. PCR products were probed with oligonucleotides specific for the unique first exon of each transcript, and RNA integrity was verified by amplification of transcripts for $beta$ -actin and PCNA (not shown). Note that a longer exposure is shown for the HCT15 5-aza-CdR time course experiment in order to emphasize differences at the earlier time points. (B) Quantitation of the results in panel A for the HCT15 cell line relative to the ubiquitously expressed transcript for PCNA.

Several of the lines in Table 1 were treated with 5-aza-CdR (Fig. 1A) to obtain evidence that the ARF promoter could be silencedby DNA methylation. The SW48, HCT116, and Raji lines were usedas controls, and ARF was expressed before drug treatment in allthree lines, although SW48 expressed more ARF RNA after treatment.INK4a was expressed before drug treatment in HCT116 cells andwas activated following 5-aza-CdR treatment in the SW48 and Rajilines (Fig. 1A). HCT15 cells, which expressed neither INK4a norARF, were monitored at various times after treatment to determineif there was differential reactivation kinetics for the two tandemlylinked genes. Induction of both transcripts occurred in a time-dependentfashion, with ARF expression slightly preceding INK4a activation,an effect most noticeable at the 34-h time point (Fig. 1A). Theresults were quantitated relative to the ubiquitously expressedtranscript for PCNA (Fig. 1B). Although ARF transcripts appearedearlier than INK4a transcripts, the INK4a transcript levels wereultimately higher than those of ARF transcripts, as shown by thecrossover of the two lines at approximately 40 h posttreatment.Our results clearly demonstrate that both transcripts can be reactivatedin tandem. Although we cannot rule out the possibility that eachtranscript is expressed from a different allele, such a situationhas not been observed in other, similar tandem promoter systems(7, 49, 74, 75).

Cloning and characterization of the human ARF promoter. We used the known sequence of exon 1 $beta$ (36) as a probe to screen a lambda genomic library to further characterize both therole of DNA methylation in suppressing ARF promoter-driven transcriptionand its regulation in general. A clone containing all of exon1 $beta$ and at least 10 kb of upstream sequence (data not shown) wasidentified, and an approximately 8.5-kb SacI fragment subclonedfrom the phage clone and the 3' end corresponded to a SacI siteat +49 (relative to the transcription start site) of the previouslypublished exon 1 $beta$ sequence (36). This fragment was subclonedfurther (see Materials and Methods) and sequenced to bp $-$ 5650relative to the previously published transcription start site(36). The sequence indicated that ARF is a TATA-less promoterand a CpG island like that seen for many other housekeeping genes.The region extending from +49 to $-$ 2678, the most CpG-rich region(encompassed by brackets in Fig. 5B), had a G/C content of 0.59and an observed-over-expected ratio of CpG of 0.78 and contained183 CpG sites, clearly meeting the established criteria for aCpG island (3, 12). Figure 2A compares the ARF promoter regionreported here with the previously analyzed INK4a promoter, alsoa CpG island (15, 18).

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FIG. 2. (A) Plots comparing the frequency of the CpG dinucleotide in the ARF promoter/exon 1 $beta$ region (top) and the INK4a/exon 1 $alpha$ region (bottom) derived from GenBank accession no. AC000048. Bent arrows are the transcription start sites, and open boxes are transcribed regions. Analysis of the regions of each promoter denoted by the brackets in terms of their CpG contents yields the following: G/C content = 0.64, observed/expected for CpG = 0.85 for ARF and G/C content = 0.54, observed/expected for CpG = 0.68 for INK4a over approximately 2,400 bp. (B) Sequence of a portion of the ARF promoter region (GenBank accession no. AF082338). The previously mapped transcription start site (36) is indicated by a bent arrow above the italicized "G" and is defined here as position +1. The positions of several potential transcription factor binding sites are underlined, as is a region homologous to other known initiator elements (Inr). Potential E2F binding sites are denoted with a line above the sequence; ( $-$ ) indicates that the consensus binding site is 5' to 3' on the bottom strand. Positions of restriction enzyme sites used in subsequent cloning steps for promoter deletion analysis are underlined, and their positions relative to the transcription start site are indicated. Downward arrows denote 5' ends of deletion constructs generated by PCR. A subset of the repetitive elements described in the text (Alu and purine-pyrimidine [Pur-Pyr]) is also shown.

The promoter region of the INK4a gene had been previously characterized (18). It is negatively regulated by pRb; however,the ARF promoter and its regulation have not been previously reported.Figure 2B indicates the locations of numerous potential transcriptionfactor binding sites. In particular, there are seven potentialbinding sites for the Sp1 transcription factor and a region homologousto the initiator element often present in TATA-less promoterssuch as this. The placement of the putative initiator relativeto the transcription start site and potential Sp1 binding sitesis similar to that for other previously described promoters (37;reviewed in reference 67). Also notable are several repetitiveelements, such as an Alu element at positions $-$ 2942 to $-$ 2695,a thymine-cytosine run from $-$ 3109 to $-$ 3056 (not shown), a guanine-thyminerun from $-$ 125 to $-$ 92, three potential AP-1 sites at $-$ 4977, $-$ 4829,and $-$ 3394 (not shown) (reviewed in reference 24), and one potentialYY1 site at $-$ 3152 (not shown) (66).

To determine if this region possessed promoter activity and to define important regulatory regions, 5'-end deletions weremade by using naturally occurring restriction enzyme sites orPCR and fused to the CAT reporter gene, and the effects were assayedin several cell lines. The results, shown in Fig. 3, indicatedthat the largest construct, to $-$ 5502 (all numbering is relativeto the transcription start site), ranged from slightly inhibitoryin COS-7 and C-33A cells to potently inhibitory in HCT116 cells.Deletion to $-$ 4690 restored high level activity in HCT116 cellsbut had a relatively minor effect in the other two lines. Thebinding site for a tissue-specific repressor protein or a silencermay reside within this region. Deletion to $-$ 3407 dramaticallyreduced ARF-driven promoter activity in HCT116 cells; however,a large increase in promoter-driven CAT activity was observedin C-33A and COS-7 cells. Deletion to $-$ 2465 reduced activity tosome extent, and further deletion to $-$ 925 caused a very modestreduction in activity in COS-7 cells but resulted in slight increasesin activity in HCT116 and C-33A cells despite deletion of twopotential Sp1 binding sites (Fig. 2B). Deletion to $-$ 776 and $-$ 331resulted in significant increases in CAT activity in all threecell lines, indicating that a repressive element may reside withinthis region. Fine deletions nearer the transcription start siteto $-$ 151, $-$ 67, $-$ 44, and $-$ 19, which delete two, three, four, andfive potential Sp1 binding sites respectively, resulted in a gradualdecline of activity in COS-7 and C-33A cells. There was a slightincrease in activity upon deletion to $-$ 44 in HCT116 cells, thereason for which is unclear; however, further deletion to $-$ 19resulted in low-level promoter activity in HCT116 cells. Overall,the effects of the various promoter deletion constructs were similarin COS-7 and C-33A cells but differed significantly from effectsin the HCT116 line. This finding may indicate a difference inthe transcription factor milieu in the colon cancer line HCT116;however, this analysis does provide clear evidence that the regionwe have cloned upstream of ARF acts as a promoter.

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FIG. 3. ARF promoter deletion analysis. The extent of each of the 5' deletions fused to the CAT reporter gene, as well as the extent of each construct relative to the transcription start site (indicated by the bent arrow), is indicated schematically at the left. Results are presented as the mean relative activity (percent acetylation/ $beta$ -galactosidase activity) for triplicate transfections into the HCT116 (A), C-33A (B), and COS-7 (C) cell lines. Error bars indicate the standard deviations (SD) from the means.

A recent study using adenoviral vectors expressing the five members of the E2F family of transcription factors indicated thatARF mRNA levels were elevated after infection with adenovirusesexpressing E2F1 and E2F2 but not E2F3 to E2F5 (9), and we havenoted several potential E2F binding sites in Fig. 2B. Good matchesto the binding site consensus TTTCCCGCC(A/T)(A/T)(A/T), foundto be optimal binding sites for E2F1 to E2F4 in a binding siteselection assay (72), were detected at $-$ 265 and +27, while poorermatches to this and the standard E2F consensus binding site TTTCGCGC(reviewed in reference 24) were detected at $-$ 249 and $-$ 69. Figure3 also indicated that these regions were important for transcriptionin all cell lines. To determine if the previously observed increasein ARF mRNA after E2F1 overexpression was modulated at the transcriptionallevel, we cotransfected various ARF reporter deletion constructswith an E2F1 expression vector or empty parental expression vector.Figure 4 indicates that the ARF promoter is highly responsiveto E2F1 (nearly 15-fold) and that the regions mediating this responsecorrelate with the locations of potential E2F binding sites. Weare at present unsure if the E2F site at +27 would be utilizedin the intact natural promoter since it is downstream of the transcriptionstart site. This will require further fine mapping experiments.An INK4a reporter construct served as a negative control and wasunaffected by E2F1 overexpression.

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FIG. 4. The ARF promoter is upregulated by E2F1 expression. Each of the ARF or INK4a promoter constructs denoted schematically at the left was cotransfected with an equal amount of an expression vector for E2F1 or empty parental expression vector. The results of duplicate transfections in the HCT116 cell line are presented as the mean fold activation with E2F1 cotransfection (activity with E2F1/activity with empty expression vector). Error bars indicate the standard deviations (SD) from the means.

Comparison of the overall activities of the ARF promoter constructs in Fig. 3 showed that the cell lines could be orderedas C-33A > COS-7 > HCT116 in terms of promoter strength, whichcorrelated with the p53 status of the lines. HCT116 contains awild-type p53 gene (47), while C-33A has a mutant p53 gene (22),and COS-7 cells express the simian virus 40 large T antigen (T-Ag),which complexes with and inactivates both p53 and pRb (reviewedin references 29 and 45). This is particularly relevant sinceit has been noted that ARF levels are elevated in cells lackingfunctional p53 (27, 52), the implication being that p53 maysuppress ARF transcription. Results of the transfections studieswere consistent with this idea, and further direct evidence forthe role of p53 in suppressing ARF at the transcriptional levelwill be presented later.

Suppression of ARF promoter activity by CpG methylation. The previous results indicated that the ARF promoter was silent in only two cell lines (HCT15 and LoVo) and that ARF transcriptioncould be activated in HCT15 cells after treatment with 5-aza-CdR.HCT15 and LoVo cells were investigated in more detail to determineif this transcriptional silence might be mediated by hypermethylationof the CpG island associated with the ARF promoter. Genomic DNAfrom these lines was digested with various methylation-sensitiverestriction enzymes and analyzed by Southern blotting (Fig. 5).The digestion pattern obtained with restriction enzymes sensitiveto CpG methylation with DNA obtained from the ARF-expressing HCT116cells was consistent with complete hypomethylation of the CpGsites examined since the high-molecular-weight SacI band of approximately8.5 kb was absent in the double digests. The exception was theAatII site, which was partially methylated in this line (Fig.5A). A similar result was obtained with normal leukocyte DNA exceptthat the AatII site was completely hypomethylated (not shown),showing that the CpG island of ARF was unmethylated in normaltissues and in HCT116 cells which expressed the ARF transcript(Table 1 and Fig. 1A). Many of the CpG sites within the promoterwere, however, hypermethylated in HCT15 cells, as indicated bythe presence of higher-molecular-weight bands, relative to theHCT116 digests, indicating the the 8.5-kb SacI fragment was onlypartially cut by the methylation-sensitive enzymes. The results,summarized in Fig. 5B and C, indicated that there was a relativelysmall region of hypermethylation at the 3' end of the ARF CpGisland which did not extend significantly beyond $-$ 450 relativeto the transcription start site.

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FIG. 5. Methylation analysis of the ARF promoter. (A) Representative Southern blots after digestion of HCT116 and HCT15 genomic DNAs with the enzymes indicated and probing with the fragment shown in panels B and C. The presence of higher-molecular-weight bands in the HCT15 digests compared to the HCT116 digests is indicative of methylation. The low level of hybridization after digestion with enzymes like HpaII and HhaI is a result of the large number of such sites, creating many small restriction fragments which hybridize poorly. (B) Schematic of the location of several of the rare-cutting methylation-sensitive restriction enzyme sites, a CpG plot of the entire sequenced region, and the transcription start site (+1). Brackets in the CpG plot indicate the boundaries used for the calculation of CpG island status. The location of the probe is indicated by the thick bar, and the methylation status at the CpG sites analyzed by restriction digest is indicated by the lollipops. (C) Blowup of the region immediately adjacent to the ARF promoter ( $-$ 930 to +49) and summary of the methylation status of CpG sites in this region as determined from blots in panel A for the HCT15 cell line. Asterisks indicate that these particular CpG sites, while partially methylated in HCT15 cells, were completely methylated in the LoVo cell line (not shown). The sizes of the fragments are indicated below the lines. A lollipop displaced below a group of restriction enzyme sites indicates that the sites were too close together to accurately determine which site was digested. (D) Analysis of the methylation sensitivity of the p( $-$ 151)19ARF promoter CAT construct after in vitro methylation and transfection into HCT116 or COS-7 cells. Results after treatment with the various methylases are presented as the mean percent activity relative to the mock-methylated control (no methylase) for triplicate transfections. Error bars represent the standard deviations.

Sensitivity of the ARF promoter to CpG methylation was further examined by in vitro methylation and transfection. The ARFconstruct containing sequences from +49 to $-$ 151 fused to the CATgene was chosen for this study since the Southern blotting studies(Fig. 5A to C) indicated that hypermethylation was confined tothe region close to the transcription start site and that thisconstruct possessed a significant degree of promoter activityin its unmethylated state. The $-$ 151 construct was methylated invitro with HpaII methylase (1 recognition site), HhaI methylase(4 recognition sites), and CpG methylase (16 recognition sites)and transfected into HCT116 and COS-7 cells. Figure 5D shows thatCpG methylase had the most repressive effect, reducing reportergene activity to 10% or less of that of the mock-methylated controlin both lines. Interestingly, methylation at the single HpaIIsite had a larger repressive effect than methylation at the fourHhaI sites. This finding may indicate that the HpaII site residesin or near the binding site of a critical transcription factor,although no matches to consensus binding sites of known transcriptionfactors were detected in this region.

ARF and INK4a promoter constructs are expression competent in all cell lines. We next determined if the expression patterns for INK4a and ARF shown in Table 1 were a result of differences in the transcriptionfactor milieu or differences in the methylation status of theendogenous gene promoter sequences. A series of ARF and INK4apromoter reporter constructs were transfected into cells witheach of the previously mentioned expression patterns. Both theARF promoter and the INK4a promoter were capable of driving expressionof the CAT gene in all cell lines regardless of whether the endogenousARF or INK4a gene was transcribed (Fig. 6). Both promoters werealso nearly equal in their overall activities when the most activeconstruct for each promoter was compared, with the exception ofthe ARF⁺ INK4a⁺ and ARF⁺ INK4a cell lines, in which the ARF promoter gave a slightly higherlevel of expression. This effect was most notable in the ARF⁺ INK4a SW48 line and may indicate that there is some differential regulationof these two promoters in some situations. There was, however,some correlation between the absolute CAT activity levels andthe activity levels of the endogenous promoters. For example,the overall activities of the ARF and INK4a CAT constructs werehighest in the ARF⁺ INK4a⁺ and ARF⁺ INK4a lines (Fig. 6A and B), while the ARF INK4a HCT15 cell line had the lowest overall promoter activity (Fig.6C). Thus, the transcription factors necessary for ARF and INK4apromoter activity are present in all cell lines, although therelative levels of these factors may vary to some extent. Theinactivity of the endogenous promoter was related to its methylationstatus. It has been shown that the ARF promoter is hypermethylatedand inactive in the HCT15 line (Fig. 1A and 5A) and the INK4apromoter is inactive and hypermethylated in the HCT15 and SW48lines (Fig. 1A; references 2 and 21). It should also be notedthat the INK4a promoter analysis presented here differed in somerespects from previously published data in that deletions beyond $-$ 654 retained relatively high activity levels (18). The reasonsfor this are unclear but may be due to differences in promoterconstruction, since our constructs contained less sequence atthe 3' end than in the previous analysis.

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FIG. 6. Comparison of activities of ARF and INK4a promoter-CAT constructs after transfection into ARF⁺ INK4a⁺ (A), ARF⁺ INK4a (B), and ARF INK4a (C) cell lines. The map of each of the reporter constructs relative to the transcription start site of each promoter (for INK4a, the 5'-most initiation site was defined as +1) is indicated at the left and the mean relative activity (percent acetylation/ $beta$ -galactosidase activity) for triplicate (duplicate for SW48 and HCT15) transfections is shown at the right. Error bars indicate the standard deviations (SD) from the means.

Regulation of the INK4a/ARF locus by p53. The above studies showed that the ARF promoter region can become de novo methylated and transcriptionally silenced; however,this appeared to be a low-frequency event in cell lines, makingit unlikely that this phenomenon would occur frequently in primarytumors. Another potential regulatory control mechanism of ARFexpression may be mediated by the tumor suppressor gene p53, sinceARF levels are elevated in cell lines lacking functional p53,implying that p53 may suppress ARF. While not rigorously quantitated,the increase in ARF expression in previous reports has rangedfrom 5- to 10-fold (18, 27, 52). Since we now had availablethe ARF promoter, we were able to test the hypothesis that p53may suppress ARF at the transcriptional level.

Initially we transfected a series of ARF and INK4a reporter deletion constructs with a fixed amount of wild-type p53 expressionvector or empty parental expression vector into the p53-mutantcell line C-33A. The results (Fig. 7) indicated that both theARF and INK4a promoters were significantly repressed and thatthe majority of the repressive effect was mediated by the regionencompassing the transcription initiation sites. A small proportionof the repressive effect also appeared to be mediated by additionalregions from $-$ 151 to $-$ 67 of the ARF promoter and $-$ 654 to $-$ 474of the INK4a promoter. The majority of the repressive effect beingmediated by the region containing the transcription start siteis entirely consistent with the proposed mechanism of p53 repression,that is, interaction with the TBP component of the TFIID complex,causing a reduction in transcriptional initiation of certain promoterswhich do not contain p53 binding sites (62). We did not detectany p53 binding sites within the sequenced region of ARF or thereported INK4a promoter sequence. It should also be noted thatalthough both promoters are TATA-less, the TBP-TFIID complex hasbeen shown to be required for transcriptional initiation at TATA-lesspromoters (5).

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FIG. 7. Mapping p53-responsive regions of the ARF and INK4a promoters. Each of the reporter constructs indicated schematically at the left of each graph was cotransfected with 1.0 µg of wild-type p53 expression vector or empty parental expression vector into the C-33A cell line. Results are presented as the mean activity for triplicate transfections relative to the transfection containing no p53 expression vector, set at 100%. Error bars represent the standard deviations (SD).

To further study the effects of p53 overexpression on the ARF and INK4a promoters, we cotransfected reporter constructs demonstratinga high degree of repression in the previous experiment ( $-$ 331 forARF and $-$ 654 for INK4a) with increasing amounts of an expressionvector encoding wild-type p53 or mutant p53 (DNA binding domain,Val-143 $right-arrow$ Ala) into both the HCT116 cell line (endogenous p53 wildtype) (47) and the C-33A cell line (endogenous p53 mutant) (22).The total amount of expression vector was held constant by additionof parental expression vector containing no cDNA (Fig. 8). Promoteractivities were repressed approximately 1.6-fold for INK4a and2.5-fold for ARF at the highest levels of wild-type p53 in theHCT116 cell line (Fig. 8A). Transfection into the C-33A line withwild-type p53 resulted in an even greater degree of repression,approximately 5.5-fold for INK4a and 17.2-fold for ARF at thehighest levels of p53 (Fig. 8A). Clear differences in the sensitivitiesof the two promoters to p53 could been seen (1.6- and 3.1-foldfor HCT116 and C-33A, respectively), indicating that the repressionwas unlikely to be a nonspecific effect of p53 overexpression.The degree of repression seen with wild-type p53 overexpression,particularly in C-33A, appears sufficient to account for the previouslyobserved differences in ARF expression between p53-expressingand -nonexpressing cell lines (18, 27, 52). Transfectionwith increasing amounts of mutant p53 resulted in an approximatelytwofold increase in the activities of both the INK4a and ARF promotersin the HCT116 cell line, with no clear difference between thetwo promoters; however, in C-33A cells a very slight increasein INK4a promoter activity was observed with increasing amountsof mutant p53, while the ARF promoter appeared not to be significantlyaffected (Fig. 8B). The differences in the effect of overexpressionof mutant p53 in HCT116 and C-33A cells were most likely due todifferences in the status of the endogenous p53 gene. Two additionalCAT reporter constructs were used as comparison and control. ACAT reporter vector driven by the human p53 gene promoter (p53proCAT)served as a negative control for the effects of p53 overexpression(Fig. 8A), and a CAT reporter plasmid containing two copies ofa consensus p53 binding site driving an E1b TATA minimal promoter[2X(p53)BSCAT] was used as a positive control for a promoter containingp53 binding sites (46) and therefore able to be activated byp53. Cotransfection of increasing amounts of wild-type p53 withthe latter CAT reporter plasmid showed that the repressive effectswere not due to nonspecific inhibition of all transcription inthese cells. Reporter gene activity (expressed as the percentacetylation) was dramatically (approximately 20-fold) increasedin both cell lines, while cotransfection with mutant p53 had littleeffect (Fig. 8C).

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FIG. 8. Effects of p53 on ARF and INK4a promoter-CAT constructs. (A) Dose-response cotransfection of wild-type p53 expression vector and p( $-$ 331)19ARF, p( $-$ 654)16INK4a, or p53proCAT promoter-CAT constructs into the HCT116 and C-33A cell lines. (B) The identical CAT reporter constructs cotransfected with increasing amounts of a mutant (Val-143 $right-arrow$ Ala) p53 expression vector. Results in panels A and B are presented as the mean activity for triplicate transfections relative to the transfection containing no p53 expression vector, set at 100%. Error bars represent the standard deviations. The total amount of expression vector was held constant by addition of parental vector containing no cDNA. (C) Representative results after transfection of a CAT reporter construct containing two copies of a consensus p53 binding site with increasing amounts of wild-type or mutant p53 expression vector into the HCT116 and C-33A cell lines. Results are presented as percent acetylation; independent experiments yielded similar results. Note that the endogenous p53 gene is wild type in HCT116 and mutant in C-33A.

The previously described experiments relied on overexpression of p53, and so we next wished to determine if similar effectson transcription could be observed under physiologic conditionsin which p53 is known to be upregulated. We chose to use the DNA-damagingdrugs CMT, an inhibitor of topoisomerase I known to induce p53in a time- and dose-dependent manner (41), and Ara-C, an S-phase-specificantimetabolite that does not directly damage DNA (53) and whichhas been shown not to induce p53 (28). The latter was used asa comparison with the CMT treatment to control for nonspecificeffects on transcription due to drug cytotoxicity and cellularinsult. The HCT116 and C-33A cell lines were used again to compareeffects on ARF ( $-$ 331) and INK4a ( $-$ 654) reporter constructs. Figure9 shows that CAT activity driven by the ARF and INK4a promoterswas less in HCT116 cells treated with CMT than in HCT116 cellstreated with Ara-C. The degree of repression was similar to thatobserved previously with the wild-type p53 expression vector inHCT116 cells (Fig. 8A). No effect on ARF and INK4a reporter activitywas observed in C-33A cells treated in a similar manner, alsoconsistent with previous experiments (Fig. 8B), indicating thatrepression of the ARF and INK4a promoters can occur at physiologiclevels of p53. The 2X(p53)BSCAT reporter plasmid served as a positivecontrol to show that the CMT treatment did indeed result in anincrease in functional wild-type p53 protein. The activity ofthis construct was activated nearly sixfold in CMT-treated HCT116cells relative to Ara-C-treated HCT116 cells but unaffected insimilarly treated C-33A cells (Fig. 9). An additional negativecontrol for the effects of drug treatment, employing the p53proCATvector used previously as a negative control for p53 overexpression(Fig. 8A), was unchanged by drug treatment in both cell lines(Fig. 9).

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FIG. 9. ARF and INK4a promoters are repressed after induction of p53 by DNA-damaging agents. The reporter constructs indicated below each graph were transfected into HCT116 (A) or C-33A (B) cells, after which cells were exposed to the indicated DNA-damaging agent (5 µM CMT or 50 µM Ara-C). After 48 h, cells were harvested for CAT assay and the protein concentration was determined for each. Results are presented as the mean relative activity (percent acetylation normalized to the protein concentration to account for small differences in toxicity) of triplicate transfections. Error bars are the standard deviations from the means. WT, wild-type; MT, mutant.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

We have cloned and characterized the promoter region of the ARF putative tumor suppressor gene and investigated suppressionof this CpG island promoter by DNA methylation. Two colon cancer-derivedcell lines had hypermethylation of the ARF promoter, althoughthis occurred infrequently in cell lines and is therefore unlikelyto be common in uncultured tumors. We have also provided functionalevidence that hypermethylation can suppress ARF promoter activity.Transfection of ARF and INK4a promoter constructs revealed thatthey were active in all cell lines tested. Activity of the endogenousgenes, however, was correlated with promoter methylation status.Transfection studies also revealed that the ARF promoter was highlyresponsive to E2F1 overexpression, in keeping with previous results(9). Studies with overexpression of both wild-type and mutantforms of p53 indicated that the ARF promoter was repressed bywild-type p53 and, unexpectedly, so was its downstream neighborINK4a, although there were clear differences in the degree ofrepression. This repression was also observable under physiologicconditions in which p53 levels are increased due to DNA damage.

Sequence analysis of the ARF promoter region revealed that it possessed many of the characteristics of a housekeeping genein that it was a CpG island and a TATA-less promoter containinga region homologous to the initiator element which is responsiblefor correctly positioning the site of transcriptional initiation(5). Deletion analysis revealed that several of the potentialSp1 binding sites, as well as potential E2F binding sites, wereimportant; however, other regions not containing recognizablebinding sites were also important. It was interesting that thelargest ARF construct was less active than smaller constructsin the HCT116 cell line and that this inhibitory activity appearedto be somewhat cell type dependent. Whether a repressor proteinbinding site is present in this region or an active silencer elementis present is currently under investigation, but such elementshave been noted previously in other promoters (77). This region,however, clearly possesses many of the features of a promoterand is capable of driving significant levels of reporter geneactivity.

Treatment of the HCT15 cell line with 5-aza-CdR combined with RT-PCR expression data was interesting in several respects.First, ARF activation preceded INK4a activation after drug treatment,and second, both transcripts could clearly be expressed at thesame time. Based on previous work and the structure of the INK4a/ARFlocus, we had predicted that a transcriptional interference modelmay be in operation and that transcripts originating from theupstream ARF promoter might reduce INK4a transcriptional initiation.It was in fact observed that INK4a levels were elevated in ARF-nullmice (27). Our results do not support a transcriptional interferencemechanism such as has been observed in other situations containingtwo promoters in tandem, where it has been shown that when theupstream promoter was active the downstream one was not, and viceversa (7, 49, 50, 74, 75). It is not clear how theINK4a/ARF situation differs from these examples except that thetwo promoters are very widely spaced (estimated at 20 kb in humans[36, 68]). We cannot rule out the possibility of allele-specifictranscription of each gene, as has been observed for imprintedgenes (reviewed in reference 10). We have no evidence for differentialmethylation of this region and have not yet detected a polymorphismin the transcribed regions of the ARF and INK4a genes in the HCT15line to allow for investigation of this possibility.

Methylation-mediated silencing of INK4a has been reported in numerous situations (14, 21, 39, 59), and so it is interestingthat its neighbor ARF appeared to only rarely be subject to suchregulation. It is believed that CpG islands may be protected fromde novo methylation by binding of the Sp1 transcription factor(35). A comparison of the ARF and INK4a CpG islands revealedthat the CpG density of the ARF CpG island (number of CpG sites/bp= 0.085) was significantly higher than the INK4a CpG island (numberof CpG sites/bp = 0.048) over a similarly sized region (bracketedregions in Fig. 2A). A more dense, or larger, CpG island may confera greater protective effect against de novo methylation. The ARFpromoter contains seven potential Sp1 sites whereas the INK4apromoter contains four potential Sp1 sites upstream of the transcriptioninitiation sites, and this may also help explain the differencesin the propensity of the two promoters to become de novo methylated.An additional influence on de novo methylation of the INK4a CpGisland may arise from transcription through the INK4a promoterregion from the upstream ARF gene. The INK4a/ARF locus providesa naturally occurring system in which to study such possible effects.

Studies of the effect of E2F expression on the ARF promoter indicated a high level of responsiveness to E2F1, an effect thatwas unlikely to be nonspecific because the stimulation correlatedwith deletion of potential E2F binding sites and had no effecton an INK4a promoter construct. This stimulation at the transcriptionallevel clearly correlated with the increased levels of ARF mRNAobserved previously with E2F overexpression (9). The significanceof this finding implies that increased levels of cellular E2F,resulting from pRb phosphorylation or mutations in the pRb pathway,would increase ARF levels, which would in turn act to increasethe levels of functional p53 (48). We speculate that in normalcells, this might account for the observed increase in p53 levelsas cells enter the cell cycle from quiescence (54). In a malignantor premalignant cell resulting from mutation in the pRb pathway,this transient increase in the level of p53 may be a mechanismto induce apoptosis since pRb dysfunction, would, unlike DNA damage,be irreparable. Such potential relationships will be the subjectof future study.

Investigation of the role of p53 in regulating ARF expression at the transcriptional level was motivated by the findings inprevious work that ARF levels were elevated approximately 5- to10-fold in p53-deficient cell lines at the protein level (27,52). Our results from the wild-type p53 dose-response transfectionsshow that the ARF promoter is repressed 3- to 17-fold at the highestlevels of wild-type p53 and that the degree of repression correlatedwith the status of the endogenous p53 gene. We attribute the mutedeffect in HCT116 cells compared to C-33A cells to the presenceof wild-type endogenous p53 in the former, which would be expectedto reduce the initial levels of reporter gene activity in thisline. Further support for the role of p53 came from dose-responsestudies utilizing a mutant form of p53. Cotransfection of mutantp53 with the ARF and INK4a reporter constructs into HCT116 resultedin an increase in activity, presumably due to heterotetramerizationwith the endogenous wild-type p53 interfering with its repressiveabilities, while in C-33A, cotransfection of the mutant form ofp53 had little to no effect.

Is the repression observed with p53 overexpression a nonspecific effect, and is it physiologically relevant? Overexpressionof p53 has been shown to repress a variety of other promoters(for the c-fos, c-jun, hsc70 [13], PCNA [38], and interleukin-6[58] genes), while other promoters are unaffected (the humanp53 gene promoter in our studies; the $beta$ -actin, c-Ha-ras, epidermalgrowth factor [6], and $beta$ 2-microglobulin [38] gene promoters).We feel that the repression of the ARF and INK4a promoters ismeaningful for several reasons. First, the degree of repressionseen with the ARF promoter was reproducibly greater than thatobserved with the INK4a promoter even though the two promotershad similar activities in the absence of added p53 and were withinthe same plasmid backbone. Second, the effects were reproduciblein two different cell lines and correlated with the status ofthe endogenous p53 gene in each line. Third, the effect of mutantp53 was selective in that promoter activity actually increasedsignificantly in the cell line in which the endogenous p53 genewas wild type, while little to no effect of mutant p53 overexpressionwas observed in the cell line containing a mutant endogenous p53gene. Lastly, a similar degree of transcriptional repression ofthe ARF and INK4a promoters was observed after induction of physiologiclevels of p53 by DNA-damaging agents in a cell line with wild-typep53 function but not in a cell line with a mutant p53 gene comparedto the p53 overexpression studies.

We were initially surprised by the effects of p53 on the INK4a reporter construct. It had been reported that the INK4a promoterwas repressed three- to fivefold by pRb overexpression and thatp53 status had no effect in a cell line containing a temperature-sensitivesimian virus 40 T-Ag. T-Ag binds to and inactivates both pRb andp53 (reviewed in reference 40), and this study concluded thatthe repressive effect observed when the T-Ag was inactivated aftershift to the nonpermissive temperature was due solely to the pRbcomponent. The effect of p53 was not directly tested (18), andso reinterpretation of both this study and others is consistentwith the notion that p53 overexpression may have a repressiveeffect on INK4a levels. For example, INK4a levels were elevatedafter transfection of the E6 oncoprotein (which specifically inactivatesp53 [reviewed in reference 40]) into a cell line with otherwisewild-type pRb and p53 function (70). Thus, we propose that bothpRb and p53 may regulate INK4a and ARF. The regulation is, however,differential, with p53 being the dominant component for ARF andpRb being the dominant component for INK4a. The effect of p53on INK4a may in fact be mediated through pRb as has been previouslyproposed (70).

The nearly 20-fold decrease in ARF-driven reporter gene activity in the C-33A cell line when wild-type p53 was overexpressedmay well be sufficient to account for the corresponding increasein ARF levels in p53-deficient cell lines that has been reportedpreviously (27, 52); however, two additional factors needto be considered: (i) the stability of the RNA and (ii) the stabilityof the protein. It has been shown that the INK4a RNA is very stable(18), although similar information is not available for theARF RNA. INK4a protein has a long half-life of at least 3 h (44),while ARF has a significantly shorter half-life of approximately90 min (78). This has important implications for our resultsbecause in order to rapidly change the level of a protein by controllingthe rate of transcription, a short-lived RNA or protein is essential.The short half-life of ARF indicates that control at the transcriptionallevel would allow for rapid changes in protein levels when p53levels are elevated under physiological situations and why lessof an effect of p53 overexpression is seen on the INK4a proteinlevel with its long half-life. We cannot rule out the possibilitythat there are other levels of regulation between ARF and p53;however, it is clear from these studies that the ARF promotercan be regulated by p53 at the transcriptional level.

Recent work has shown that the role of ARF in p53-dependent cell cycle checkpoint control is mediated by its binding to theMDM2 proto-oncogene accompanied by an increase in functional p53levels and an enhancement of the capability of p53 to transactivatepromoters containing p53 binding sites (48). Based on this studyand the work presented here, we propose the existence of an autoregulatoryfeedback loop which allows for tight controls over the levelsof p53 in normal cells (Fig. 10). In this model, ARF expressionand binding to MDM2 results in an increase in functional p53 levels,allowing for either cell cycle arrest or induction of apoptosis.The increased levels of p53 will then feed back on the ARF promoter,resulting in a down-regulation of ARF transcription and concomitantdecreases in ARF protein. This will then free MDM2 to bind top53 and reduce its levels by targeting it for degradation. Additionalelements of this pathway, such as the factors regulating MDM2and ARF levels, and the role of E2F and pRb, will no doubt bethe focus of much future study given that the INK4a/ARF locusnow stands firmly at the crossroads of two of the most importantcell cycle regulatory pathways.

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FIG. 10. Proposed regulatory cycle controlling cellular p53 levels mediated by p53, MDM2, and ARF. Interaction between MDM2 and ARF results in increased degradation of MDM2 (78) (shown by light stipple) and an increase in functional p53 (upward arrow) (48). This then represses ARF (×) and activates MDM2 (large arrow) transcription (1, 76). Elevated levels of MDM2 and decreased levels of ARF then promote degradation of p53 (shown by light stipple) and continue the cycle as shown. E2F levels may be one of the outside influences on the cycle.

	ACKNOWLEDGMENTS

This work was supported by grants R35 CA 49758-09 and T32 CA 09320-15 from the National Institutes of Health.

We thank Felicidad Gonzales for technical assistance and Richard Ambinder for providing cell lines and plasmids.

	FOOTNOTES

^* Corresponding author. Mailing address: The University of Southern California, Norris Comprehensive Cancer Center, 1441 EastlakeAve., MS 83, Los Angeles, CA 90033. Phone: (323) 865-0816. Fax:(323) 865-0102. E-mail: jones_p{at}froggy.hsc.usc.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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3. Bird, A. 1986. CpG-Rich islands and the function of DNA methylation. Nature 321:209-213[Medline].

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