The Essential Cofactor TRRAP Recruits the Histone Acetyltransferase hGCN5 to c-Myc

doi:10.1128/MCB.20.2.556-562.2000

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by McMahon, S. B.
	Articles by Cole, M. D.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by McMahon, S. B.
	Articles by Cole, M. D.

Previous Article | Next Article

Molecular and Cellular Biology, January 2000, p. 556-562, Vol. 20, No. 2
0270-7306/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The Essential Cofactor TRRAP Recruits the Histone Acetyltransferase hGCN5 to c-Myc

Steven B. McMahon, Marcelo A. Wood, and Michael D. Cole^*

Department of Molecular Biology, Princeton University, Princeton, New Jersey 08544-1014

Received 22 June 1999/Returned for modification 28 July 1999/Accepted 22 October 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The c-Myc protein functions as a transcription factor to facilitate oncogenic transformation; however, the biochemical andgenetic pathways leading to transformation remain undefined. Wedemonstrate here that the recently described c-Myc cofactor TRRAPrecruits histone acetylase activity, which is catalyzed by thehuman GCN5 protein. Since c-Myc function is inhibited by recruitmentof histone deacetylase activity through Mad family proteins, theseopposing biochemical activities are likely to be responsible forthe antagonistic biological effects of c-Myc and Mad on targetgenes and ultimately on cellulartransformation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The c-Myc oncoprotein functions as a transcription factor and exerts a variety of biological effects in both normal and malignantcells (reviewed in reference 12). c-Myc functions include theability to transform primary rodent fibroblasts in cooperationwith an activated allele of p21^H-ras, the induction of apoptosis in growth factor-deprived cells,the ability to block the terminal differentiation of cells inseveral in vitro differentiation models, and the ability to promoteS-phase induction when expressed in otherwise quiescent cells(reviewed in reference 4). The most widely accepted model ofc-Myc function suggests that c-Myc-Max heterodimers bind to CACGTGconsensus sites within regulatory regions of specific cellulargenes (11). In support of this model, the C-terminal DNA bindingdomain (DBD) of c-Myc is essential for all its biological activities(25, 35, 40). Many potential c-Myc target genes have beenreported (32), although none of the proposed targets appearto mediate the potent effects of c-Myc on cell cycle progression(reviewed in reference 10).

c-Myc function is antagonized by another heterodimeric transcription factor complex containing one of the Mad family proteinsin association with Max (1, 20, 23, 47, 50). Mad-Maxdimers block c-Myc-Max function by recruitment of either of twolarge nuclear proteins, mSin3A or mSin3B (2, 36), which inturn recruit one of the two histone deacetylases, HDAC1 and HDAC2(18, 22, 51). Since Myc-Max and Mad-Max dimers are reportedto have indistinguishable DNA binding specificities (1, 50),current models suggest that repression of c-Myc function by theMad-Max-mSin3-HDAC complex results from the deacetylation of nucleosomalhistones at shared target sites within the genome (12).

Studies from our lab and others suggest that defining the function of the c-Myc N terminus may provide insight into the roleof c-Myc in oncogenic transformation and normal cell cycle progression(6, 14, 25, 29). While the precise biochemical mechanismremains unknown, the c-Myc N terminus has been shown to be requiredfor transcriptional activation (21). All biological activitiesof c-Myc also require an evolutionarily conserved block of approximately20 amino acids referred to as MbII (6, 35, 40). However,deletion of MbII has no deleterious effect on transactivationby c-Myc as measured in conventional reporter gene assays (6).We have recently found that the MbII domain is required to recruita novel nuclear cofactor called TRRAP and that TRRAP is essentialfor the oncogenic activity of c-Myc (29).

Traditionally, the activation domains of transcription factors have been thought to function either by mediating the recruitmentof the basal transcriptional machinery or by the recruitment ofcomplexes capable of altering nucleosomal organization (49).We recently found that the Saccharomyces cerevisiae ortholog ofTRRAP, TRA1p, is a component of the SAGA complex (34), whichregulates transcription through chromatin remodeling. Within themultiprotein SAGA complex the only known catalytic subunit isGCN5p (15), which mediates the acetylation of histone tails,resulting in an open chromatin configuration and increased transcription.Several distinct mammalian complexes with characteristics similarto those of the S. cerevisiae SAGA complex have recently beenidentified (28, 30, 46). The present study was undertakento determine whether c-Myc, through its association with TRRAP,recruits a mammalian histone acetylase complex, thereby providinga potential mechanism for the antagonistic functions of c-Myc-Maxand Mad-Max dimers on target gene expression and cellulartransformation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Purification of HeLa cell nuclear proteins interacting with the c-Myc N terminus. FLAG epitope-tagged GAL4 and GAL4-c-Myc fusion proteins were produced by baculovirus infection of insect cells as previouslydescribed (29). Nuclear extracts from HeLa cells were generatedand then mixed with the baculovirus-produced proteins as describedelsewhere (29).

Immunoprecipitation. 293 cell lysates were prepared as described elsewhere (29) and subjected to immunoprecipitation with rabbit antisera directedagainst c-Myc (N262; Santa Cruz Biotechnology), Max (C-17; SantaCruz Biotechnology), or hGCN5 (generous gift from Nickolai Barlevand Shelley Berger) (8) or with a mouse monoclonal antibodyagainst c-Myc (C-33; Santa Cruz Biotechnology). Precipitated proteinswere either resolved by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) on an 8% gel and immunoblottedby using standard techniques or subjected to a histone acetyltransferase(HAT) assay as describedbelow.

HAT assay. c-Myc-associated HeLa cell proteins or 293 immunoprecipitates were assayed for HAT activity essentially as described elsewhere(7). Purified histones (type II-A; Sigma) and radiolabeledacetyl coenzyme A (acetyl-CoA) (TRK688; Amersham) were purchasedfrom the suppliersindicated.

Transformation assay. Primary rat embryo fibroblasts were transfected as described previously (29). Transfections included an activated alleleof p21^H-ras (1 µg) in conjunction with the equal amounts of the c-Myc expressionvectors indicated. Cells were maintained in Dulbecco modifiedEagle medium (Gibco BRL) with 4% fetal calf serum for 2 weeks,at which time transformed foci werecounted.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Since c-Myc oncoprotein function can be antagonized by Mad and the recruitment of histone deacetylases, we were interestedin determining whether c-Myc itself could recruit HAT activity.In particular, we focused on the N-terminal domain of c-Myc, whichis required for cell transformation but not for DNA binding. Wehave recently described an approach for the affinity purificationof nuclear cofactors associated with the c-Myc N terminus (29).Briefly, a FLAG epitope-tagged protein containing murine c-Myc(amino acids 1 to 262) fused to the GAL4 DBD was produced by baculovirusinfection of insect cells and then used as an affinity reagentto isolate c-Myc N-terminus-interacting complexes from HeLa cellnuclear extracts. This protocol was previously used for the isolationof the novel c-Myc cofactor TRRAP from prefractionated nuclearextracts. In the present experiments, unfractionated nuclear extractswere mixed with the FLAG-GAL4-c-Myc fusion protein and then immunoprecipitatedwith antibodies to the FLAG epitope. Precipitates were washed,and the captured proteins were eluted from the antibody by incubationwith FLAG peptide. This protocol allows the isolation of GAL4-c-Mycand any associated proteins in their native configuration suchthat they can be assayed for both protein composition and biochemicalactivity. An epitope-tagged protein containing only the GAL4 DBDserved as a control. Nuclear proteins from HeLa cells which wererecruited to the c-Myc N terminus were assayed for HAT activityby assessing their ability to transfer radiolabeled acetyl groupsfrom acetyl-CoA to purified histones (Fig. 1). The results ofthis assay firmly establish that the c-Myc N terminus recruitsHeLa nuclear protein(s) capable of significant histone acetylation(Fig. 1), whereas the control affinity matrix (FLAG-GAL4) recruitsnegligible activity in comparison.

View larger version (24K):
[in this window]
[in a new window]

FIG. 1. The c-Myc N terminus recruits a HAT. (A) FLAG epitope-tagged GAL4 DBD or a FLAG epitope-tagged GAL4 DBD-c-Myc (amino acids 1 to 262) fusion was used as an affinity matrix to isolate proteins from HeLa cell nuclear extracts. (B) Proteins recruited by each matrix were incubated with purified histones in the presence of radiolabeled acetyl-CoA. Following filter binding and washing, the degree of histone acetylation in each sample was quantitated by scintillation counting. Assays were performed in triplicate. Values for individual samples after subtraction of background are reported.

Among the mammalian nuclear cofactors with well-documented histone acetylase activity is the ortholog of the yeast proteinGCN5p, termed hGCN5 in humans (45). We have recently shown thatin yeast, TRA1p is a component of the GCN5p-containing SAGA complex(34). This observation prompted an examination of whether hGCN5could account for the HAT activity associated with the c-Myc Nterminus. Western blots of affinity-purified proteins were probedwith anti-hGCN5 serum, revealing that the c-Myc N terminus formeda specific interaction with hGCN5 from HeLa cell nuclear extracts(Fig. 2A, lower panel). The hGCN5 protein detected by the antiserummigrates with an apparent molecular mass of 100 kDa, consistentwith the full-length form of the protein. While some investigatorshave reported the existence of a 50-kDa form of hGCN5 (termedhGCN5-S) (8, 37), no such species was apparent in our studies.The specificity of the hGCN5 interaction with c-Myc was demonstratedby the absence of detectable hGCN5 in eluates from GAL4 DBD affinitypurification. As previously reported, the c-Myc N terminus alsospecifically recruits the nuclear cofactor TRRAP (Fig. 2A, upperpanel). By comparing the signal for hGCN5 in our captured materialto the signal obtained from a known quantity of the starting extract(HeLa nuclear extracts [Fig. 2B]), we have determined that lessthan 0.1% of the total hGCN5 available is recruited in our invitro binding reactions. However, this estimate may be artificiallylower than the actual percentage of hGCN5 recruited into the c-Myc-TRRAPcomplex, since the in vitro purification scheme requires thatthe complex remain stable through both a 16-h binding reactionand an extensive series of wash steps.

View larger version (32K):
[in this window]
[in a new window]

FIG. 2. The c-Myc N terminus recruits the HAT hGCN5. (A) Proteins captured by the GAL4 DBD or GAL4 DBD-c-Myc fusion were resolved by SDS-PAGE (8% gel) and immunoblotted for either the c-Myc cofactor TRRAP (A) or the recently described mammalian HAT hGCN5 (B). Antibodies to hGCN5 were the generous gift from Nickolai Barlev and Shelley Berger. Numbers at left (in kilodaltons) indicate positions of size markers. (B) Western blotting for hGCN5 was performed with HeLa cell nuclear extracts and whole-cell lysates from 293 cells.

The in vitro binding of hGCN5 to the c-Myc N terminus prompted an examination of whether this interaction could be observedin vivo with endogenous proteins. c-Myc-Max heterodimers wereimmunoprecipitated from 293 cell lysates by using antibodies specificfor Max (Fig. 3A, lower panel). Western blots of the precipitatesshowed that hGCN5 specifically associates with the c-Myc-Max dimer(Fig. 3A, middle panel). Control antiserum did not precipitateeither c-Myc or hGCN5 (Fig. 3A, lane 1). TRRAP was also specificallycoprecipitated with the c-Myc-Max heterodimers as previously demonstrated(Fig. 3A, upper panel). Identical results were obtained when anti-c-Mycantibodies were used for immunoprecipitation (Fig. 3B).

View larger version (38K):
[in this window]
[in a new window]

FIG. 3. Myc family oncoproteins recruit hGCN5 in human cells. (A) 293 cells were lysed under nondenaturing conditions, and c-Myc-Max dimers were immunoprecipitated with antisera against Max (lanes 2 and 3). A parallel precipitation was performed with nonimmune rabbit serum (NRS) as a control (lane 1). Precipitated proteins were resolved by SDS-PAGE (8% gel) and subjected to immunoblotting for either c-Myc (lower panel), hGCN5 (middle panel), or TRRAP (upper panel). Numbers at the left (in kilodaltons) indicate positions of size markers. The position of the heavy-chain polypeptide from the precipitating antibody is indicated (Ig). (B) 293 cells were lysed and subjected to immunoprecipitation with either a control monoclonal antibody (ø) or a monoclonal antibody directed against c-Myc. Immunoprecipitates (i.p.) were blotted and probed for TRRAP (upper panel) and hGCN5 (lower panel). (C) 293 cells were transiently transfected with a cytomegalovirus-driven expression vector encoding FLAG epitope-tagged versions of either wild-type (wt) murine N-Myc (lane 2) or a mutant lacking amino acids 100 to 116 of the MbII domain (lane 3). Following transfection, cells were lysed as for panel A, immunoprecipitations were performed with anti-FLAG antibody; precipitates were resolved by SDS-PAGE and Western blotted for either the FLAG epitope (lower panel) or hGCN5 (upper panel). Mock transfected 293 cells served as a control (lane 1).

Recruitment of hGCN5 to c-Myc is presumed to be mediated by TRRAP, since TRRAP and GCN5 exist in the SAGA complex in S. cerevisiaewhere no Myc protein is present. We have previously demonstratedthat recruitment of TRRAP to the transactivation domain of Mycfamily proteins requires the highly conserved MbII domain (29;S. B. McMahon et al., unpublished data). TRRAP-mediated recruitmentof hGCN5 to Myc family proteins should therefore require the presenceof MbII. To test this hypothesis, 293 cells were transiently transfectedwith expression vectors encoding FLAG epitope-tagged versionsof either wild-type or MbII-deleted N-Myc. The N-Myc protein appearsto have biological activities indistinguishable from those ofc-Myc in terms of transformation potential and transactivation(S. B. McMahon and M. D. Cole, unpublished observations). Followinglysis, these proteins were immunoprecipitated and the precipitateswere analyzed by Western blotting (Fig. 3C). In keeping with aTRRAP-dependent mechanism of hGCN5 recruitment, hGCN5 is recruitedonly to wild-type N-Myc and not to the mutant of N-Myc lackingMbII (Fig. 3C, upper panel). Probing for the common FLAG epitoperevealed that both wild-type and mutant proteins were expressedand precipitated in similar quantities (Fig. 3C, lowerpanel).

We next addressed whether c-Myc-associated HAT activity could be observed by direct immunoprecipitation of endogenous c-Mycfrom human cells. For this study, lysates prepared from serum-stimulated293 cells were subjected to immunoprecipitation by antibodiesdirected against c-Myc, Max, or hGCN5. Precipitates were assayedfor HAT activity, and the results are displayed in Fig. 4. Precipitationof c-Myc, either directly or as a dimer with Max, resulted incoprecipitation of significant HAT activity relative to controlprecipitates (Fig. 4). As expected, direct precipitation of hGCN5also resulted in significant HAT activity.

View larger version (23K):
[in this window]
[in a new window]

FIG. 4. The c-Myc oncoprotein associates with HAT activity in vivo. Immunoprecipitation of 293 cell lysates for either c-Myc, Max, or hGCN5 were subjected to an in vitro HAT assay in the presence of purified histones and radiolabeled acetyl-CoA. For each precipitation, lysate was prepared from a single confluent 15-cm-diameter dish of serum-stimulated 293 cells. Precipitations contained approximately 4 mg of total protein and were conducted in triplicate. Bars represent average values (± standard error).

The experiments above demonstrate an in vivo association between the c-Myc N terminus, hGCN5, and TRRAP, but they do not resolvewhether hGCN5 is bound to c-Myc directly or through TRRAP. S.cerevisiae TRA1p copurifies with the SAGA complex which includesGCN5p, yet there is no ortholog of c-Myc in yeast. Thus, it seemedlikely that human TRRAP would also exist in a complex with hGCN5independent of c-Myc and that the binding of TRRAP to the c-MycN terminus would be responsible for recruitment of the hGCN5 proteinto the complex. To distinguish between these possibilities, hGCN5was precipitated from lysates prepared from 293 cells, and theprecipitates were probed for hGCN5 (Fig. 5A, lower panel) or TRRAP(Fig. 5A, upper panel). Immunoprecipitation of hGCN5 results inthe specific coprecipitation of TRRAP, whereas parallel sampleswith control nonimmune serum showed no precipitation of eitherhGCN5 or TRRAP. Probing of these precipitates with antisera specificfor c-Myc revealed no detectable c-Myc protein in the hGCN5-TRRAPcomplex (Fig. 5B), despite the presence of readily detectablec-Myc in 293 lysates when immunoprecipitated directly with anti-Mycantibodies. Coprecipitation of hGCN5 and TRRAP has also been observedin murine fibroblasts that have been rendered genetically deficientfor c-Myc (data not shown). The absence of detectable c-Myc proteinin the immunoprecipitates suggests that hGCN5 and TRRAP preexistin a complex in mammalian cells, that their interaction does notrequire c-Myc, and that only a small fraction of the hGCN5-TRRAPcomplex contains c-Myc. In support of this conclusion is the observationthat the HAT activity recruited to the c-Myc N terminus representsless than 0.1% of the total hGCN5-dependent HAT activity in HeLanuclear extracts in our in vitro binding reactions (Fig. 1 and2).

View larger version (25K):
[in this window]
[in a new window]

FIG. 5. In vivo association of hGCN5 and TRRAP in the absence of c-Myc. (A) Aliquots of 293 cell lysates were either electrophoresed directly (lane 1) or subjected to immunoprecipitation with nonimmune rabbit serum (NRS; lane 2) or anti-hGCN5 (lane 3). Proteins were resolved by SDS-PAGE (8% gel) and immunoblotted for TRRAP (upper panel) or hGCN5 (lower panel). Numbers at the left (in kilodaltons) indicate positions of molecular weight markers. (B) 293 cell lysates were subjected to immunoprecipitation with antibodies specific for hGCN5 (lane 2), c-Myc (lane 4), or species-matched, nonimmune sera (lanes 1 and 3). Precipitated proteins were resolved by SDS-PAGE (8% gel) and immunoblotted for c-Myc. The position of the heavy-chain polypeptide from the precipitating antibody is indicated (Ig).

We recently demonstrated that recruitment of TRRAP to c-Myc is essential for transformation of mammalian cells. Coupling thisobservation with the evidence reported here that TRRAP recruitshGCN5 to c-Myc suggested the possibility that recruitment of hGCN5is the essential function of TRRAP in c-Myc-mediated transformation.To test this hypothesis, the HAT domain of hGCN5 was directlyfused to a mutant of c-Myc which is defective for TRRAP recruitment.This fusion protein was then assayed for its potential to transformprimary rat embryo fibroblasts in cooperation with an activatedallele of p21^H-ras. As evident in Fig. 6A, wild-type c-Myc is a potent transformingagent, while the MbII deletion mutant (which fails to recruitTRRAP) is completely defective for transformation. Fusion of thehGCN5 HAT domain to this transformation-defective c-Myc mutantprovides a partial rescue of its transforming potential (Fig.6A and C). To ensure that this partial rescue was due to the HATactivity of hGCN5, specific point mutations were introduced inthree amino acids known to be essential for the enzymatic functionof GCN5 proteins (44). Introduction of these mutations blockedtransformation by the fusion protein (Fig. 6A), suggesting thatthe loss of TRRAP recruitment can be rescued only by direct recruitmentof an enzymatically active HAT domain. Further support for a rolefor hGCN5 in c-Myc-mediated transformation comes from studiesin which a dominant negative mutant of hGCN5 (which carries thesame mutations in the catalytic domain as those described above)blocks transformation by c-Myc (Fig. 6B). Expression of wild-typehGCN5 in this assay had no significant effect.

View larger version (45K):
[in this window]
[in a new window]

FIG. 6. Partial rescue of a nontransforming c-Myc mutant by direct fusion to hGCN5. (A) Primary rat embryo fibroblasts were transfected with expression vectors for an activated allele of p21^H-ras and one of the c-Myc constructs schematized at the left. The c-Myc constructs encoded either wild-type mouse c-Myc or a deletion mutant of this protein lacking 17 amino acids from the MbII domain. In addition, two fusion proteins were generated between the c-Myc MbII domain deletion mutant and the catalytic domain of hGCN5 (amino acids 370 to 837). For the first of these fusions, wild-type hGCN5 sequences were fused to c-Myc $Delta$ MbII. The second fusion contained three single amino acid substitutions within the hGCN5 HAT domain (as indicated by x's). These mutations have been shown previously to block both HAT activity and transcriptional activation when introduced into the corresponding residues of S. cerevisiae GCN5. The critical bromodomain of hGCN5 (labeled B) was also included in these fusion proteins. Transforming potential of each of these proteins was determined by examining cells approximately 2 weeks posttransfection. Transforming potential was estimated based on both the total number of transformed foci generated with a given protein and the size of the individual foci obtained. bHLH-LZ, basic helix-loop-helix leucine zipper. (B) A transformation assay was performed as for panel A except that full-length versions of hGCN5 were coexpressed with c-Myc. Both wild-type and catalytically inactive forms of hGCN5 were assayed for their effect on c-Myc mediated transformation. (C) Representative foci obtained by transfection of rat embryo fibroblasts with p21^H-ras and either wild-type c-Myc (left) or the MbII mutant-hGCN5 fusion protein (right).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

All of the biological functions of c-Myc require a unique N-terminal domain whose biochemical function has only recently beendetermined (29). We show here that one function of this domainis to recruit the HAT hGCN5, which presumably modifies nucleosomalpackaging at specific chromosomal targets. The recruitment ofhGCN5 by c-Myc is mediated by the recently described nuclear cofactorTRRAP (29). TRRAP and hGCN5 are contained in a complex whichassociates with the c-Myc N terminus in vivo and after in vitroreconstitution. Furthermore, immunoprecipitation of endogenousc-Myc results in the copurification of a potent HAT activity fromhuman cells. Finally, we show that hGCN5 exists in a complex withTRRAP in vivo that is independent of any association through c-Myc.Since the binding of TRRAP and hGCN5 to Myc is dependent on theessential N-terminal domain, MbII, it appears likely that therecruitment of the TRRAP-hGCN5 complex may also be essential forc-Myc biologicalactivities.

Many recent studies have demonstrated that the acetylation of histones is a critical step in gene activation, and severaltranscriptional cofactors have been shown to have HAT activity(3, 9, 31, 39, 48). Mad-Max heterodimers inhibit thetransforming activity of c-Myc-Max heterodimers, while both heterodimersreportedly possess the same DNA binding specificity (1, 20,23, 47, 50). In addition, overexpression of Mad leads toa dose-dependent decrease in the ability of c-Myc to transactivatereporter genes (1, 47). Mad-mediated inhibition of c-Mycfunction requires an interaction between Mad and the mSin3 adapterprotein (2, 36), and this complex subsequently recruits theHDAC family of histone deacetylases (18, 22, 51). The currentmodel suggests that Mad-Max dimers bind to c-Myc-Max target siteswithin the genome, recruiting the mSin3-HDAC complex which inturn deacetylates nearby histones, resulting in a closed chromatinconfiguration at essential c-Myc target genes (11). The resultspresented in this study provide a biochemical basis for the antagonisticeffects of Myc and Mad by demonstrating that c-Myc recruits theHAT hGCN5, whose activity would be directly opposed by the recruitmentof the histone deacetylase HDAC by Mad (Fig. 7).

View larger version (31K):
[in this window]
[in a new window]

FIG. 7. Model of the opposing biochemical functions of c-Myc and Mad. Mad family proteins dimerize with Max and repress the expression of c-myc and max target genes, thereby blocking c-Myc function. Mad-mediated repression requires the recruitment of a multiprotein complex containing histone deacetylases of the HDAC family. The demonstration here that c-Myc, through its essential cofactor TRRAP, recruits the mammalian HAT hGCN5 suggests a potential biochemical basis for antagonistic biological functions of c-Myc and Mad. In this model, c-Myc-Max heterodimers activate transcription of target genes by recruitment of TRRAP and a HAT such as hGCN5. HAT activity results in nucleosomal remodeling at target gene loci, allowing more efficient transcription. Following displacement of Myc-Max dimers from their cognate DNA recognition element, Mad-Max dimers recruit deacetylase activity to these sites, which in turn removes the acetyl groups from histones in nearby nucleosomes. This process facilitates chromatin condensation and consequently transcriptional repression.

In S. cerevisiae, TRA1p is a component of the macromolecular SAGA complex (34). At least four distinct mammalian counterpartsof the SAGA complex have now been described (28, 30, 46);two of them, TFTC and STAGA, contain the full-length form of hGCN5.TFTC and STAGA can be distinguished based on the presence andabsence, respectively, of the TAF_II100 protein. Our preliminaryresults indicate that the hGCN5-TRRAP complex recruited to thec-Myc N terminus (as defined in Fig. 2) lacks TAF_II100 (data notshown). While this result suggests that the hGCN5 complex recruitedby c-Myc is STAGA-like, it remains possible that c-Myc recruitsan hGCN5 complex which is distinct from those described to date.Moreover, in S. cerevisiae, TRA1 is essential for viability (34)whereas the GCN5 gene is not (13, 27). This observation suggeststhat the histone acetylase hGCN5 may not be the only criticalactivity recruited to c-Myc by TRRAP. In support of this suggestion,TRA1p has been reported to be a component of a second multiproteintranscriptional regulatory complex designated NuA4 (16). TheNuA4 complex lacks GCN5p but contains another HAT, ESA1p (16);like TRA1, ESA1 is essential for growth of S. cerevisiae (38).The interaction of TRRAP with potential human orthologs of ESA1pis currently under investigation. In addition, it has recentlybeen reported that in human cells, TRRAP is a component of a largemultiprotein complex which includes the hGCN5 homolog PCAF (42).Our failure to detect PCAF in our c-Myc complexes (data not shown)presumably results from the low expression level of PCAF in theHeLa and 293 cells used in our study. To date, no functional distinctionshave been found between the closely related hGCN5 and PCAF proteins,and current data suggest that TRRAP can enter complexes containingeither of these HATs (this study and reference 42). In addition,it remains possible that TRRAP recruits other HAT proteins toc-Myc.

The finding that a majority of the TRRAP-hGCN5 complex lacks c-Myc suggests that this complex also plays a role in the activityof transcription factors other than c-Myc. In support of this,we have recently reported that TRRAP is recruited to the transactivationdomain of the E2F1 transcription factor (29). Intriguingly,E2F1 activity, like that of c-Myc, is antagonized by the HDACfamily of histone deacetylases (5, 24, 26). Furthermore,another component of the SAGA complex (ADA3) binds to the nuclearretinoic acid receptor (43). Since TRA1p, GCN5p, and ADA3p/NGG1pare all components of SAGA in yeast (15, 19, 33, 34),it seems likely that mammalian TRRAP will associate not only withhGCN5 but also with the other components of the mammalian SAGAcomplex. This complex is presumably available for recruitmentby many mammalian transcription factors in addition to c-Myc.

The partial genetic rescue of transformation by direct fusion of the hGCN5 catalytic domain to the $Delta$ MbII mutant of c-Myc suggeststhat at least some portion of the essential role of TRRAP as acofactor for c-Myc relies on its ability to recruit hGCN5 or asimilar HAT to c-Myc target genes. The finding that only a partialrescue is achieved by direct recruitment of a HAT may result fromthe artificial context in which the HAT domain is located in thefusion protein, potentially resulting in suboptimal HAT activityor slightly altered substrate specificity. An alternative explanationfor the partial rescue is that the c-Myc N terminus provides essentialfunctions other than recruitment of the TRRAP-hGCN5 complex. Insupport of this hypothesis, we have recently isolated a secondchromatin remodeling complex which is recruited to the c-Myc Nterminus and which may function in concert with the HAT activityrecruited by TRRAP (46a).

c-Myc is capable of both activation and repression of distinct target genes (32). An implication of the results presentedhere is that targets of the c-Myc-TRRAP-hGCN5 complex should berestricted to the subset of genes activated by c-Myc. This conclusionis based on current models of chromatin reorganization, whichsuggest that acetylation of core histone by proteins such as hGCN5results in an open configuration, thereby allowing more efficienttranscription (41). Thus, it is perplexing that MbII deletionmutations in c-Myc that fail to bind TRRAP do not have reducedtransactivation activity in most transient reporter assays (6).One explanation is that transiently transfected DNA is not packagedinto a chromatin configuration that is responsive to the recruitmentof hGCN5-mediated acetylation of histones. As most assays of therole of MbII in transactivation have been performed with episomalplasmids as targets, they may not represent an accurate assessmentof the true role of MbII in transactivation by c-Myc.

Current models of HAT protein activity suggest that one hypothesis for the role of hGCN5 in c-Myc's activities might be dueto the relaxing of chromatin packaging at target genes followinghistone acetylation by hGCN5. Alternatively, hGCN5 may be recruitedto this complex to acetylate nonhistone proteins such as c-Mycitself. This second scenario has ample precedence, for example,with the acetylation of p53 protein by p300, which results inincreased p53 DNA binding activity (17). If hGCN5 acetylatesnonhistone proteins when recruited into the c-Myc-TRRAP complex,a simple histone-based model of functional activity may requirereevaluation.

	ACKNOWLEDGMENTS

We are grateful to Shelley Berger and Nickolai Barlev of the Wistar Institute for generously providing antibodies to humanGCN5 and to Elizabeth Moran for advice regarding histone acetylationassays. We also thank Penny Rushton for excellent technicalassistance.

S.B.M. is a Special Fellow of the Leukemia Society ofAmerica.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Biology, Princeton University, Princeton, NJ 08544-1014. Phone:(609) 258-5936. Fax: (609) 258-2759. E-mail: mcole{at}molbio.princeton.edu.

Present address: The Wistar Institute, Philadelphia, PA 19104-4268.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ayer, D. E., L. Kretzner, and R. N. Eisenman. 1993. Mad: a heterodimeric partner for max that antagonizes myc transcriptional activity. Cell 72:211-222[CrossRef][Medline].

2. Ayer, D. E., Q. A. Lawrence, and R. N. Eisenman. 1995. Mad-Max transcriptional repression is mediated by ternary complex formation with mammalian homologs of yeast repressor Sin3. Cell 80:767-776[CrossRef][Medline].

3. Bannister, A. J., and T. Kouzarides. 1996. The CBP co-activator is a histone acetyltransferase. Nature 384:641-643[CrossRef][Medline].

4. Bouchard, C., P. Staller, and M. Eilers. 1998. Control of cell proliferation by Myc. Trends Cell Biol. 8:202-206[CrossRef][Medline].

5. Brehm, A., E. A. Miska, D. J. McCance, J. L. Reid, A. J. Bannister, and T. Kouzarides. 1998. Retinoblastoma protein recruits histone deacetylase to repress transcription. Nature 391:597-601[CrossRef][Medline].

6. Brough, D. E., T. J. Hofmann, K. B. Ellwood, R. A. Townley, and M. D. Cole. 1995. An essential domain of the c-Myc protein interacts with a nuclear factor that is also required for E1A-mediated transformation. Mol. Cell. Biol. 15:1536-1544[Abstract].

7. Brownell, J. E., and C. D. Allis. 1995. An activity gel assay detects a single, catalytically active histone acetyltransferase subunit in Tetrahymena macronuclei. Proc. Natl. Acad. Sci. USA 92:6364-6368[Abstract/Free Full Text].

8. Candau, R., P. A. Moore, L. Wang, N. Barlev, C. Y. Ying, C. A. Rosen, and S. L. Berger. 1996. Identification of human proteins functionally conserved with yeast putative adaptors ADA2 and GCN5. Mol. Cell. Biol. 16:593-602[Abstract].

9. Chen, H., R. J. Lin, R. L. Schiltz, D. Chakravarti, A. Nash, L. Nagy, M. L. Privalsky, Y. Nakatani, and R. M. Evans. 1997. Nuclear receptor coactivator ACTR is a novel histone acetyltransferase and forms a multimeric complex with P/CAF and CBP/p300. Cell 90:569-580[CrossRef][Medline].

10. Cole, M. D., and S. B. McMahon. 1999. The Myc oncoprotein: a critical evaluation of transactivation and target gene regulation. Oncogene 18:2916-2924[CrossRef][Medline].

11. Dang, C. V. 1999. c-Myc target genes involved in cell growth, apoptosis, and metabolism. Mol. Cell. Biol. 19:1-11[Free Full Text].

12. Facchini, L. M., and L. Z. Penn. 1998. The molecular role of Myc in growth and transformation: recent discoveries lead to new insights. FASEB J. 12:633-651[Abstract/Free Full Text].

13. Georgakopoulos, T., and G. Thireos. 1992. Two distinct yeast transcriptional activators require the function of the GCN5 protein to promote normal levels of transcription. EMBO J. 11:4145-4152[Medline].

14. Goruppi, S., S. Gustincich, C. Brancolini, W. M. F. Lee, and C. Schneider. 1994. Dissection of c-myc domains involved in S phase induction in NIH3T3 fibroblasts. Oncogene 9:1537-1544[Medline].

15. Grant, P. A., L. Duggan, J. Cote, S. M. Roberts, J. E. Brownell, R. Candau, R. Ohba, T. Owen-Hughes, C. D. Allis, F. Winston, S. L. Berger, and J. L. Workman. 1997. Yeast Gcn5 functions in two multisubunit complexes to acetylate nucleosomal histones: characterization of an Ada complex and the SAGA (Spt/Ada) complex. Genes Dev. 11:1640-1650[Abstract/Free Full Text].

16. Grant, P. A., D. Schieltz, M. G. Pray-Grant, J. R. Yates III, and J. L. Workman. 1998. The ATM-related cofactor Tra1 is a component of the purified SAGA complex. Mol. Cell 2:863-867[CrossRef][Medline].

17. Gu, W., and R. G. Roeder. 1997. Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain. Cell 90:595-605[CrossRef][Medline].

18. Hassig, C. A., T. C. Fleischer, A. N. Billin, S. L. Schreiber, and D. E. Ayer. 1997. Histone deacetylase activity is required for full transcriptional repression by mSin3A. Cell 89:341-347[CrossRef][Medline].

19. Horiuchi, J., N. Silverman, G. A. Marcus, and L. Guarente. 1995. ADA3, a putative transcriptional adaptor, consists of two separable domains and interacts with ADA2 and GCN5 in a trimeric complex. Mol. Cell. Biol. 15:1203-1209[Abstract].

20. Hurlin, P. J., C. Queva, P. J. Koskinen, E. Steingrimsson, D. E. Ayer, N. G. Copeland, N. A. Jenkins, and R. N. Eisenman. 1995. Mad3 and Mad4: novel Max-interacting transcriptional repressors that suppress c-myc dependent transformation and are expressed during neural and epidermal differentiation. EMBO J. 14:223-232.

21. Kato, G. J., J. Barrett, M. Villa-Garcia, and C. V. Dang. 1990. An amino-terminal c-Myc domain required for neoplastic transformation activates transcription. Mol. Cell. Biol. 10:5914-5920[Abstract/Free Full Text].

22. Laherty, C. D., W. M. Yang, J. M. Sun, J. R. Davie, E. Seto, and R. N. Eisenman. 1997. Histone deacetylases associated with the mSin3 corepressor mediate Mad transcriptional repression. Cell 89:349-356[CrossRef][Medline].

23. Lahoz, E. G., L. Xu, N. Schreiber-Agus, and R. A. DePinho. 1994. Suppression of Myc, but not E1a, transformation activity by Max-associated proteins, Mad and Mxil. Proc. Natl. Acad. Sci. USA 91:5503-5507[Abstract/Free Full Text].

24. Luo, R. X., A. A. Postigo, and D. C. Dean. 1998. Rb interacts with histone deacetylase to repress transcription. Cell 92:463-473[CrossRef][Medline].

25. MacGregor, D., L. H. Li, and E. B. Ziff. 1996. Dominant negative mutants of Myc inhibit cooperation of both Myc and adenovirus serotype-5 E1A with Ras. J. Cell. Physiol. 167:95-105[CrossRef][Medline].

26. Magnaghi-Jaulin, L., R. Groisman, I. Naguibneva, P. Robin, S. Lorain, J. P. Le Villain, F. Troalen, D. Trouche, and A. Harel-Bellan. 1998. Retinoblastoma protein represses transcription by recruiting a histone deacetylase. Nature 391:601-605[CrossRef][Medline].

27. Marcus, G., N. Silverman, S. Berger, J. Horiuchi, and L. Guarente. 1994. Functional similarity and physical association between GCN5 and ADA2: putative transcriptional adaptors. EMBO J. 13:4807-4815[Medline].

28. Martinez, E., T. K. Kunda, J. Fu, and R. G. Roeder. 1998. A human SPT3-TAF_II31-GCN5-L acetylase complex distinct from transcription factor IID. J. Biol. Chem. 273:23781-23785[Abstract/Free Full Text].

29. McMahon, S. B., H. A. VanBuskirk, K. A. Dugan, T. D. Copeland, and M. D. Cole. 1998. The novel ATM-related protein TRRAP is an essential cofactor for the c-Myc and E2F oncoproteins. Cell 94:363-374[CrossRef][Medline].

30. Ogryzko, V. V., T. Kotani, X. Zhang, R. L. Schiltz, T. Howard, J. Quin, and Y. Nakatani. 1998. Histone-like TAFs within the PCAF histone acetylase complex. Cell 94:35-44[CrossRef][Medline].

31. Ogryzko, V. V., R. L. Schiltz, V. Russanova, B. H. Howard, and Y. Nakatani. 1996. The transcriptional coactivators p300 and CBP are histone acetyltransferases. Cell 87:953-959[CrossRef][Medline].

32. Peters, M. A., and E. J. Taparowsky. 1998. Target genes and cellular regulators of the Myc transcription complex. Crit. Rev. Eukaryot. Gene Expr. 8:277-296[Medline].

33. Saleh, A., V. Lang, R. Cook, and C. J. Brandl. 1997. Identification of native complexes containing the yeast coactivator/repressor proteins NGG1/ADA3 and ADA2. J. Biol. Chem. 272:5571-5578[Abstract/Free Full Text].

34. Saleh, A., D. Schieltz, N. Ting, S. B. McMahon, D. W. Litchfield, J. R. Yates III, S. P. Lees-Miller, M. D. Cole, and C. J. Brandl. 1998. Tra1p is a component of the yeast ADA/SPT transcriptional regulatory complexes. J. Biol. Chem. 273:26559-26570[Abstract/Free Full Text].

35. Sarid, J., T. D. Halazonetis, W. Murphy, and P. Leder. 1987. Evolutionarily conserved regions of the human c-myc protein can be uncoupled from transforming activity. Proc. Natl. Acad. Sci. USA 84:170-173[Abstract/Free Full Text].

36. Schreiber-Agus, N., L. Chin, K. Chen, R. Torres, G. Rao, P. Guida, A. I. Skoultchi, and R. A. DePinho. 1995. An amino-terminal domain of Mxi1 mediates anti-Myc oncogenic activity and interacts with a homolog of the yeast transcriptional repressor SIN3. Cell 80:777-786[CrossRef][Medline].

37. Smith, E. R., J. M. Belote, R. L. Schiltz, X.-J. Yang, P. A. Moore, S. L. Berger, Y. Nakatani, and C. D. Allis. 1998. Cloning of Drosophila GCN5: conserved features among metazoan GCN5 family members. Nucleic Acids Res. 26:2948-2954[Abstract/Free Full Text].

38. Smith, E. R., A. Eisen, W. Gu, M. Sattah, A. Pannuti, J. Zhou, R. G. Cook, J. C. Lucchesi, and C. D. Allis. 1998. ESA1 is a histone acetyltransferase that is essential for growth in yeast. Proc. Natl. Acad. Sci. USA 95:3561-3565[Abstract/Free Full Text].

39. Spencer, T. E., G. Jenster, M. M. Burcin, C. D. Allis, J. Zhou, C. A. Mizzen, N. J. McKenna, S. A. Onate, S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1997. Steroid receptor coactivator-1 is a histone acetyltransferase. Nature 389:194-198[CrossRef][Medline].

40. Stone, J., T. DeLange, G. Ramsay, E. Jakobovits, J. M. Bishop, H. Varmus, and W. Lee. 1987. Definition of regions in human c-myc that are involved in transformation and nuclear localization. Mol. Cell. Biol. 7:1697-1709[Abstract/Free Full Text].

41. Struhl, K. 1998. Histone acetylation and transcriptional regulatory mechanisms. Genes Dev. 12:599-606[Free Full Text].

42. Vassilev, A., J. Yamauchi, T. Kotani, C. Prives, M. L. Avantaggiati, J. Qin, and Y. Nakatani. 1998. The 400 kDa subunit of the PCAF histone acetylase complex belongs to the ATM superfamily. Mol. Cell 2:869-875[CrossRef][Medline].

43. vom Baur, E., M. Harbers, S. J. Um, A. Benecke, P. Chambon, and R. Losson. 1998. The yeast Ada complex mediates the ligand-dependent activation function AF-2 of retinoid X and estrogen receptors. Genes Dev. 12:1278-1289[Abstract/Free Full Text].

44. Wang, L., L. Liu, and S. L. Berger. 1998. Critical residues for histone acetylation by GCN5, functioning in Ada and SAGA complexes, are also required for transcriptional function in vivo. Genes Dev. 12:640-653[Abstract/Free Full Text].

45. Wang, L., C. Mizzen, C. Ying, R. Candau, N. Barlev, J. Brownell, C. D. Allis, and S. L. Berger. 1997. Histone acetyltransferase activity is conserved between yeast and human GCN5 and is required for complementation of growth and transcriptional activation. Mol. Cell. Biol. 17:519-527[Abstract].

46. Wieczorek, E., M. Brand, X. Jacq, and L. Tora. 1998. Function of TAF(II)-containing complex without TBP in transcription by RNA polymerase II. Nature 393:187-191[CrossRef][Medline].

46a. Wood, M. A., S. B. McMahon, and M. D. Cole. An ATPase/helicase complex is an essential cofactor for oncogenic transformation by c-Myc. Mol. Cell, in press.

47. Wu, S., A. Pena, A. Korcz, D. R. Soprano, and K. J. Soprano. 1996. Overexpression of Mxi1 inhibits the induction of the human ornithine decarboxylase gene by the Myc/Max protein complex. Oncogene 12:621-629[Medline].

48. Yang, X.-J., V. V. Ogryzko, J. Nishikawa, B. H. Howard, and Y. Nakatani. 1996. A p300/CBP-associated factor that competes with the adenoviral oncoprotein E1A. Nature 382:319-324[CrossRef][Medline].

49. Zawel, L., and D. Reinberg. 1995. Common themes in assembly and function of eukaryotic transcription complexes. Annu. Rev. Biochem. 64:533-561[CrossRef][Medline].

50. Zervos, A., J. Gyuris, and R. Brent. 1993. Mxi1, a protein that specifically interacts with Max to bind Myc-Max recognition sites. Cell 72:223-232[CrossRef][Medline].

51. Zhang, Y., R. Iratni, H. Erdjument-Bromage, P. Tempst, and D. Reinberg. 1997. Histone deacetylases and Sap18, a novel polypeptide, are components of a human Sin3 complex. Cell 89:357-364[CrossRef][Medline].

This article has been cited by other articles:

ten Berge, D., Brugmann, S. A., Helms, J. A., Nusse, R. (2008). Wnt and FGF signals interact to coordinate growth with cell fate specification during limb development. Development 135: 3247-3257 [Abstract] [Full Text]
Liu, X., Vorontchikhina, M., Wang, Y.-L., Faiola, F., Martinez, E. (2008). STAGA Recruits Mediator to the MYC Oncoprotein To Stimulate Transcription and Cell Proliferation. Mol. Cell. Biol. 28: 108-121 [Abstract] [Full Text]
DeRan, M., Pulvino, M., Greene, E., Su, C., Zhao, J. (2008). Transcriptional Activation of Histone Genes Requires NPAT-Dependent Recruitment of TRRAP-Tip60 Complex to Histone Promoters during the G1/S Phase Transition. Mol. Cell. Biol. 28: 435-447 [Abstract] [Full Text]
Kenneth, N. S., Ramsbottom, B. A., Gomez-Roman, N., Marshall, L., Cole, P. A., White, R. J. (2007). TRRAP and GCN5 are used by c-Myc to activate RNA polymerase III transcription. Proc. Natl. Acad. Sci. USA 104: 14917-14922 [Abstract] [Full Text]
Jason Collier, J., Zhang, P., Pedersen, K. B., Burke, S. J., Haycock, J. W., Scott, D. K. (2007). c-Myc and ChREBP regulate glucose-mediated expression of the L-type pyruvate kinase gene in INS-1-derived 832/13 cells. Am. J. Physiol. Endocrinol. Metab. 293: E48-E56 [Abstract] [Full Text]
Knoepfler, P. S. (2007). Myc Goes Global: New Tricks for an Old Oncogene. Cancer Res. 67: 5061-5063 [Abstract] [Full Text]
Cowling, V. H., Cole, M. D. (2007). The Myc Transactivation Domain Promotes Global Phosphorylation of the RNA Polymerase II Carboxy-Terminal Domain Independently of Direct DNA Binding. Mol. Cell. Biol. 27: 2059-2073 [Abstract] [Full Text]
Secombe, J., Li, L., Carlos, L., Eisenman, R. N. (2007). The Trithorax group protein Lid is a trimethyl histone H3K4 demethylase required for dMyc-induced cell growth. Genes Dev. 21: 537-551 [Abstract] [Full Text]
Rickards, B., Flint, S. J., Cole, M. D., LeRoy, G. (2007). Nucleolin Is Required for RNA Polymerase I Transcription In Vivo. Mol. Cell. Biol. 27: 937-948 [Abstract] [Full Text]
Cowling, V. H., Chandriani, S., Whitfield, M. L., Cole, M. D. (2006). A Conserved Myc Protein Domain, MBIV, Regulates DNA Binding, Apoptosis, Transformation, and G2 Arrest.. Mol. Cell. Biol. 26: 4226-4239 [Abstract] [Full Text]
Mo, H., Henriksson, M. (2006). Identification of small molecules that induce apoptosis in a Myc-dependent manner and inhibit Myc-driven transformation. Proc. Natl. Acad. Sci. USA 103: 6344-6349 [Abstract] [Full Text]
Gause, M., Eissenberg, J. C., MacRae, A. F., Dorsett, M., Misulovin, Z., Dorsett, D. (2006). Nipped-A, the Tra1/TRRAP Subunit of the Drosophila SAGA and Tip60 Complexes, Has Multiple Roles in Notch Signaling during Wing Development.. Mol. Cell. Biol. 26: 2347-2359 [Abstract] [Full Text]
Patel, J. H., McMahon, S. B. (2006). Targeting of Miz-1 Is Essential for Myc-mediated Apoptosis. J. Biol. Chem. 281: 3283-3289 [Abstract] [Full Text]
Hooker, C. W., Hurlin, P. J. (2006). Of Myc and Mnt. J. Cell Sci. 119: 208-216 [Abstract] [Full Text]
Zhang, X.-y., DeSalle, L. M., Patel, J. H., Capobianco, A. J., Yu, D., Thomas-Tikhonenko, A., McMahon, S. B. (2005). Metastasis-associated protein 1 (MTA1) is an essential downstream effector of the c-MYC oncoprotein. Proc. Natl. Acad. Sci. USA 102: 13968-13973 [Abstract] [Full Text]
Perini, G., Diolaiti, D., Porro, A., Della Valle, G. (2005). In vivo transcriptional regulation of N-Myc target genes is controlled by E-box methylation. Proc. Natl. Acad. Sci. USA 102: 12117-12122 [Abstract] [Full Text]
Loo, L. W. M., Secombe, J., Little, J. T., Carlos, L.-S., Yost, C., Cheng, P.-F., Flynn, E. M., Edgar, B. A., Eisenman, R. N. (2005). The Transcriptional Repressor dMnt Is a Regulator of Growth in Drosophila melanogaster. Mol. Cell. Biol. 25: 7078-7091 [Abstract] [Full Text]
Awasthi, S., Sharma, A., Wong, K., Zhang, J., Matlock, E. F., Rogers, L., Motloch, P., Takemoto, S., Taguchi, H., Cole, M. D., Luscher, B., Dittrich, O., Tagami, H., Nakatani, Y., McGee, M., Girard, A.-M., Gaughan, L., Robson, C. N., Monnat, R. J. Jr., Harrod, R. (2005). A Human T-Cell Lymphotropic Virus Type 1 Enhancer of Myc Transforming Potential Stabilizes Myc-TIP60 Transcriptional Interactions. Mol. Cell. Biol. 25: 6178-6198 [Abstract] [Full Text]
Huang, A., Ho, C. S.W., Ponzielli, R., Barsyte-Lovejoy, D., Bouffet, E., Picard, D., Hawkins, C. E., Penn, L. Z. (2005). Identification of a Novel c-Myc Protein Interactor, JPO2, with Transforming Activity in Medulloblastoma Cells. Cancer Res. 65: 5607-5619 [Abstract] [Full Text]
Tominaga, K., Kirtane, B., Jackson, J. G., Ikeno, Y., Ikeda, T., Hawks, C., Smith, J. R., Matzuk, M. M., Pereira-Smith, O. M. (2005). MRG15 Regulates Embryonic Development and Cell Proliferation. Mol. Cell. Biol. 25: 2924-2937 [Abstract] [Full Text]
Liu, L., Li, L., Rao, J. N., Zou, T., Zhang, H. M., Boneva, D., Bernard, M. S., Wang, J.-Y. (2005). Polyamine-modulated expression of c-myc plays a critical role in stimulation of normal intestinal epithelial cell proliferation. Am. J. Physiol. Cell Physiol. 288: C89-C99 [Abstract] [Full Text]
Patel, J. H., Du, Y., Ard, P. G., Phillips, C., Carella, B., Chen, C.-J., Rakowski, C., Chatterjee, C., Lieberman, P. M., Lane, W. S., Blobel, G. A., McMahon, S. B. (2004). The c-MYC Oncoprotein Is a Substrate of the Acetyltransferases hGCN5/PCAF and TIP60. Mol. Cell. Biol. 24: 10826-10834 [Abstract] [Full Text]
Blum, K. A., Lozanski, G., Byrd, J. C. (2004). Adult Burkitt leukemia and lymphoma. Blood 104: 3009-3020 [Abstract] [Full Text]
Marinkovic, D., Marinkovic, T., Kokai, E., Barth, T., Moller, P., Wirth, T. (2004). Identification of novel Myc target genes with a potential role in lymphomagenesis. Nucleic Acids Res 32: 5368-5378 [Abstract] [Full Text]
Mao, D. Y. L., Barsyte-Lovejoy, D., Ho, C. S. W., Watson, J. D., Stojanova, A., Penn, L. Z. (2004). Promoter-binding and repression of PDGFRB by c-Myc are separable activities. Nucleic Acids Res 32: 3462-3468 [Abstract] [Full Text]
Le Guezennec, X., Vriend, G., Stunnenberg, H. G. (2004). Molecular Determinants of the Interaction of Mad with the PAH2 Domain of mSin3. J. Biol. Chem. 279: 25823-25829 [Abstract] [Full Text]
Grinberg, A. V., Hu, C.-D., Kerppola, T. K. (2004). Visualization of Myc/Max/Mad Family Dimers and the Competition for Dimerization in Living Cells. Mol. Cell. Biol. 24: 4294-4308 [Abstract] [Full Text]
Thomas-Tikhonenko, A., Viard-Leveugle, I., Dews, M., Wehrli, P., Sevignani, C., Yu, D., Ricci, S., el-Deiry, W., Aronow, B., Kaya, G., Saurat, J.-H., French, L. E. (2004). Myc-Transformed Epithelial Cells Down-Regulate Clusterin, Which Inhibits Their Growth in Vitro and Carcinogenesis in Vivo. Cancer Res. 64: 3126-3136 [Abstract] [Full Text]
Greenwald, R. J., Tumang, J. R., Sinha, A., Currier, N., Cardiff, R. D., Rothstein, T. L., Faller, D. V., Denis, G. V. (2004). E{micro}-BRD2 transgenic mice develop B-cell lymphoma and leukemia. Blood 103: 1475-1484 [Abstract] [Full Text]
Yang, X.-J. (2004). The diverse superfamily of lysine acetyltransferases and their roles in leukemia and other diseases. Nucleic Acids Res 32: 959-976 [Abstract] [Full Text]
Herceg, Z., Li, H., Cuenin, C., Shukla, V., Radolf, M., Steinlein, P., Wang, Z.-Q. (2003). Genome-wide analysis of gene expression regulated by the HAT cofactor Trrap in conditional knockout cells. Nucleic Acids Res 31: 7011-7023 [Abstract] [Full Text]
Pal, S., Yun, R., Datta, A., Lacomis, L., Erdjument-Bromage, H., Kumar, J., Tempst, P., Sif, S. (2003). mSin3A/Histone Deacetylase 2- and PRMT5-Containing Brg1 Complex Is Involved in Transcriptional Repression of the Myc Target Gene cad. Mol. Cell. Biol. 23: 7475-7487 [Abstract] [Full Text]
Adhikary, S., Peukert, K., Karsunky, H., Beuger, V., Lutz, W., Elsasser, H.-P., Moroy, T., Eilers, M. (2003). Miz1 Is Required for Early Embryonic Development during Gastrulation. Mol. Cell. Biol. 23: 7648-7657 [Abstract] [Full Text]
Lu, F., Zhou, J., Wiedmer, A., Madden, K., Yuan, Y., Lieberman, P. M. (2003). Chromatin Remodeling of the Kaposi's Sarcoma-Associated Herpesvirus ORF50 Promoter Correlates with Reactivation from Latency. J. Virol. 77: 11425-11435 [Abstract] [Full Text]
Hennemann, H., Vassen, L., Geisen, C., Eilers, M., Moroy, T. (2003). Identification of a Novel Kruppel-associated Box Domain Protein, Krim-1, That Interacts with c-Myc and Inhibits Its Oncogenic Activity. J. Biol. Chem. 278: 28799-28811 [Abstract] [Full Text]
Horikawa, I., Barrett, J. C. (2003). Transcriptional regulation of the telomerase hTERT gene as a target for cellular and viral oncogenic mechanisms. Carcinogenesis 24: 1167-1176 [Abstract] [Full Text]
Oliver, T. G., Grasfeder, L. L., Carroll, A. L., Kaiser, C., Gillingham, C. L., Lin, S. M., Wickramasinghe, R., Scott, M. P., Wechsler-Reya, R. J. (2003). Transcriptional profiling of the Sonic hedgehog response: A critical role for N-myc in proliferation of neuronal precursors. Proc. Natl. Acad. Sci. USA 100: 7331-7336 [Abstract] [Full Text]
Liu, X., Tesfai, J., Evrard, Y. A., Dent, S. Y. R., Martinez, E. (2003). c-Myc Transformation Domain Recruits the Human STAGA Complex and Requires TRRAP and GCN5 Acetylase Activity for Transcription Activation. J. Biol. Chem. 278: 20405-20412 [Abstract] [Full Text]
Levens, D. L. (2003). Reconstructing MYC. Genes Dev. 17: 1071-1077 [Full Text]
Orian, A., van Steensel, B., Delrow, J., Bussemaker, H. J., Li, L., Sawado, T., Williams, E., Loo, L. W.M., Cowley, S. M., Yost, C., Pierce, S., Edgar, B. A., Parkhurst, S. M., Eisenman, R. N. (2003). Genomic binding by the Drosophila Myc, Max, Mad/Mnt transcription factor network. Genes Dev. 17: 1101-1114 [Abstract] [Full Text]
Schorl, C., Sedivy, J. M. (2003). Loss of Protooncogene c-Myc Function Impedes G1 Phase Progression Both before and after the Restriction Point. Mol. Biol. Cell 14: 823-835 [Abstract] [Full Text]
Mu, Z. M., Yin, X. Y., Prochownik, E. V. (2002). Pag, a Putative Tumor Suppressor, Interacts with the Myc Box II Domain of c-Myc and Selectively Alters Its Biological Function and Target Gene Expression. J. Biol. Chem. 277: 43175-43184 [Abstract] [Full Text]
Knoepfler, P. S., Cheng, P. F., Eisenman, R. N. (2002). N-myc is essential during neurogenesis for the rapid expansion of progenitor cell populations and the inhibition of neuronal differentiation. Genes Dev. 16: 2699-2712 [Abstract] [Full Text]
Eberhardy, S. R., Farnham, P. J. (2002). Myc Recruits P-TEFb to Mediate the Final Step in the Transcriptional Activation of the cad Promoter. J. Biol. Chem. 277: 40156-40162 [Abstract] [Full Text]
Watson, J. D., Oster, S. K., Shago, M., Khosravi, F., Penn, L. Z. (2002). Identifying Genes Regulated in a Myc-dependent Manner. J. Biol. Chem. 277: 36921-36930 [Abstract] [Full Text]
Park, S. W., Li, J., Loh, H. H., Wei, L.-N. (2002). A Novel Signaling Pathway of Nitric Oxide on Transcriptional Regulation of Mouse kappa Opioid Receptor Gene. J. Neurosci. 22: 7941-7947 [Abstract] [Full Text]
Cong, Y.-S., Wright, W. E., Shay, J. W. (2002). Human Telomerase and Its Regulation. Microbiol. Mol. Biol. Rev. 66: 407-425 [Abstract] [Full Text]
Ard, P. G., Chatterjee, C., Kunjibettu, S., Adside, L. R., Gralinski, L. E., McMahon, S. B. (2002). Transcriptional Regulation of the mdm2 Oncogene by p53 Requires TRRAP Acetyltransferase Complexes. Mol. Cell. Biol. 22: 5650-5661 [Abstract] [Full Text]
Nikiforov, M. A., Chandriani, S., O'Connell, B., Petrenko, O., Kotenko, I., Beavis, A., Sedivy, J. M., Cole, M. D. (2002). A Functional Screen for Myc-Responsive Genes Reveals Serine Hydroxymethyltransferase, a Major Source of the One-Carbon Unit for Cell Metabolism. Mol. Cell. Biol. 22: 5793-5800 [Abstract] [Full Text]
Vieyra, D., Loewith, R., Scott, M., Bonnefin, P., Boisvert, F.-M., Cheema, P., Pastyryeva, S., Meijer, M., Johnston, R. N., Bazett-Jones, D. P., McMahon, S., Cole, M. D., Young, D., Riabowol, K. (2002). Human ING1 Proteins Differentially Regulate Histone Acetylation. J. Biol. Chem. 277: 29832-29839 [Abstract] [Full Text]
James, L., Eisenman, R. N. (2002). Myc and Mad bHLHZ domains possess identical DNA-binding specificities but only partially overlapping functions invivo. Proc. Natl. Acad. Sci. USA 99: 10429-10434 [Abstract] [Full Text]
Tarte, K., De Vos, J., Thykjaer, T., Zhan, F., Fiol, G., Costes, V., Reme, T., Legouffe, E., Rossi, J.-F., Shaughnessy, J. Jr, Orntoft, T. F., Klein, B. (2002). Generation of polyclonal plasmablasts from peripheral blood B cells: a normal counterpart of malignant plasmablasts. Blood 100: 1113-1122 [Abstract] [Full Text]
Nikiforov, M. A., Chandriani, S., Park, J., Kotenko, I., Matheos, D., Johnsson, A., McMahon, S. B., Cole, M. D. (2002). TRRAP-Dependent and TRRAP-Independent Transcriptional Activation by Myc Family Oncoproteins. Mol. Cell. Biol. 22: 5054-5063 [Abstract] [Full Text]
Flinn, E. M., Wallberg, A. E., Hermann, S., Grant, P. A., Workman, J. L., Wright, A. P. H. (2002). Recruitment of Gcn5-containing Complexes during c-Myc-dependent Gene Activation. STRUCTURE AND FUNCTION ASPECTS. J. Biol. Chem. 277: 23399-23406 [Abstract] [Full Text]
Soucek, L., Jucker, R., Panacchia, L., Ricordy, R., Tato, F., Nasi, S. (2002). Omomyc, a Potential Myc Dominant Negative, Enhances Myc-induced Apoptosis. Cancer Res. 62: 3507-3510 [Abstract] [Full Text]
Levens, D. (2002). Disentangling the MYC web. Proc. Natl. Acad. Sci. USA 99: 5757-5759 [Full Text]
Dawson, S., Apcher, S., Mee, M., Higashitsuji, H., Baker, R., Uhle, S., Dubiel, W., Fujita, J., Mayer, R. J. (2002). Gankyrin Is an Ankyrin-repeat Oncoprotein That Interacts with CDK4 Kinase and the S6 ATPase of the 26 S Proteasome. J. Biol. Chem. 277: 10893-10902 [Abstract] [Full Text]
Park, J., Wood, M. A., Cole, M. D. (2002). BAF53 Forms Distinct Nuclear Complexes and Functions as a Critical c-Myc-Interacting Nuclear Cofactor for Oncogenic Transformation. Mol. Cell. Biol. 22: 1307-1316 [Abstract] [Full Text]
Yagi, K., Furuhashi, M., Aoki, H., Goto, D., Kuwano, H., Sugamura, K., Miyazono, K., Kato, M. (2002). c-myc Is a Downstream Target of the Smad Pathway. J. Biol. Chem. 277: 854-861 [Abstract] [Full Text]
Prescott, J. E., Osthus, R. C., Lee, L. A., Lewis, B. C., Shim, H., Barrett, J. F., Guo, Q., Hawkins, A. L., Griffin, C. A., Dang, C. V. (2001). A Novel c-Myc-responsive Gene, JPO1, Participates in Neoplastic Transformation. J. Biol. Chem. 276: 48276-48284 [Abstract] [Full Text]
Eberhardy, S. R., Farnham, P. J. (2001). c-Myc Mediates Activation of the cad Promoter via a Post-RNA Polymerase II Recruitment Mechanism. J. Biol. Chem. 276: 48562-48571 [Abstract] [Full Text]
Satou, A., Taira, T., Iguchi-Ariga, S. M. M., Ariga, H. (2001). A Novel Transrepression Pathway of c-Myc. RECRUITMENT OF A TRANSCRIPTIONAL COREPRESSOR COMPLEX TO c-Myc BY MM-1, A c-Myc-BINDING PROTEIN. J. Biol. Chem. 276: 46562-46567 [Abstract] [Full Text]
Yin, X.-Y., Grove, L., Datta, N. S., Katula, K., Long, M. W., Prochownik, E. V. (2001). Inverse Regulation of Cyclin B1 by c-Myc and p53 and Induction of Tetraploidy by Cyclin B1 Overexpression. Cancer Res. 61: 6487-6493 [Abstract] [Full Text]
Eisenman, R. N. (2001). Deconstructing Myc. Genes Dev. 15: 2023-2030 [Full Text]
Bouchard, C., Dittrich, O., Kiermaier, A., Dohmann, K., Menkel, A., Eilers, M., Luscher, B. (2001). Regulation of cyclin D2 gene expression by the Myc/Max/Mad network: Myc-dependent TRRAP recruitment and histone acetylation at the cyclin D2 promoter. Genes Dev. 15: 2042-2047 [Abstract] [Full Text]
Frank, S. R., Schroeder, M., Fernandez, P., Taubert, S., Amati, B. (2001). Binding of c-Myc to chromatin mediates mitogen-induced acetylation of histone H4 and gene activation. Genes Dev. 15: 2069-2082 [Abstract] [Full Text]
Park, J., Kunjibettu, S., McMahon, S. B., Cole, M. D. (2001). The ATM-related domain of TRRAP is required for histone acetyltransferase recruitment and Myc-dependent oncogenesis. Genes Dev. 15: 1619-1624 [Abstract] [Full Text]
Brown, C. E., Howe, L., Sousa, K., Alley, S. C., Carrozza, M. J., Tan, S., Workman, J. L. (2001). Recruitment of HAT Complexes by Direct Activator Interactions with the ATM-Related Tra1 Subunit. Science 292: 2333-2337 [Abstract] [Full Text]
Xu, D., Popov, N., Hou, M., Wang, Q., Bjorkholm, M., Gruber, A., Menkel, A. R., Henriksson, M. (2001). Switch from Myc/Max to Mad1/Max binding and decrease in histone acetylation at the telomerase reverse transcriptase promoter during differentiation of HL60 cells. Proc. Natl. Acad. Sci. USA 98: 3826-3831 [Abstract] [Full Text]
Washburn, B. K., Esposito, R. E. (2001). Identification of the Sin3-Binding Site in Ume6 Defines a Two-Step Process for Conversion of Ume6 from a Transcriptional Repressor to an Activator in Yeast. Mol. Cell. Biol. 21: 2057-2069

1.	Ayer, D. E., L. Kretzner, and R. N. Eisenman. 1993. Mad: a heterodimeric partner for max that antagonizes myc transcriptional activity. Cell 72:211-222[CrossRef][Medline].
2.	Ayer, D. E., Q. A. Lawrence, and R. N. Eisenman. 1995. Mad-Max transcriptional repression is mediated by ternary complex formation with mammalian homologs of yeast repressor Sin3. Cell 80:767-776[CrossRef][Medline].
3.	Bannister, A. J., and T. Kouzarides. 1996. The CBP co-activator is a histone acetyltransferase. Nature 384:641-643[CrossRef][Medline].
4.	Bouchard, C., P. Staller, and M. Eilers. 1998. Control of cell proliferation by Myc. Trends Cell Biol. 8:202-206[CrossRef][Medline].
5.	Brehm, A., E. A. Miska, D. J. McCance, J. L. Reid, A. J. Bannister, and T. Kouzarides. 1998. Retinoblastoma protein recruits histone deacetylase to repress transcription. Nature 391:597-601[CrossRef][Medline].
6.	Brough, D. E., T. J. Hofmann, K. B. Ellwood, R. A. Townley, and M. D. Cole. 1995. An essential domain of the c-Myc protein interacts with a nuclear factor that is also required for E1A-mediated transformation. Mol. Cell. Biol. 15:1536-1544[Abstract].
7.	Brownell, J. E., and C. D. Allis. 1995. An activity gel assay detects a single, catalytically active histone acetyltransferase subunit in Tetrahymena macronuclei. Proc. Natl. Acad. Sci. USA 92:6364-6368[Abstract/Free Full Text].
8.	Candau, R., P. A. Moore, L. Wang, N. Barlev, C. Y. Ying, C. A. Rosen, and S. L. Berger. 1996. Identification of human proteins functionally conserved with yeast putative adaptors ADA2 and GCN5. Mol. Cell. Biol. 16:593-602[Abstract].
9.	Chen, H., R. J. Lin, R. L. Schiltz, D. Chakravarti, A. Nash, L. Nagy, M. L. Privalsky, Y. Nakatani, and R. M. Evans. 1997. Nuclear receptor coactivator ACTR is a novel histone acetyltransferase and forms a multimeric complex with P/CAF and CBP/p300. Cell 90:569-580[CrossRef][Medline].
10.	Cole, M. D., and S. B. McMahon. 1999. The Myc oncoprotein: a critical evaluation of transactivation and target gene regulation. Oncogene 18:2916-2924[CrossRef][Medline].
11.	Dang, C. V. 1999. c-Myc target genes involved in cell growth, apoptosis, and metabolism. Mol. Cell. Biol. 19:1-11[Free Full Text].
12.	Facchini, L. M., and L. Z. Penn. 1998. The molecular role of Myc in growth and transformation: recent discoveries lead to new insights. FASEB J. 12:633-651[Abstract/Free Full Text].
13.	Georgakopoulos, T., and G. Thireos. 1992. Two distinct yeast transcriptional activators require the function of the GCN5 protein to promote normal levels of transcription. EMBO J. 11:4145-4152[Medline].
14.	Goruppi, S., S. Gustincich, C. Brancolini, W. M. F. Lee, and C. Schneider. 1994. Dissection of c-myc domains involved in S phase induction in NIH3T3 fibroblasts. Oncogene 9:1537-1544[Medline].
15.	Grant, P. A., L. Duggan, J. Cote, S. M. Roberts, J. E. Brownell, R. Candau, R. Ohba, T. Owen-Hughes, C. D. Allis, F. Winston, S. L. Berger, and J. L. Workman. 1997. Yeast Gcn5 functions in two multisubunit complexes to acetylate nucleosomal histones: characterization of an Ada complex and the SAGA (Spt/Ada) complex. Genes Dev. 11:1640-1650[Abstract/Free Full Text].
16.	Grant, P. A., D. Schieltz, M. G. Pray-Grant, J. R. Yates III, and J. L. Workman. 1998. The ATM-related cofactor Tra1 is a component of the purified SAGA complex. Mol. Cell 2:863-867[CrossRef][Medline].
17.	Gu, W., and R. G. Roeder. 1997. Activation of p53 sequence-specific DNA binding by acetylation of the p53 C-terminal domain. Cell 90:595-605[CrossRef][Medline].
18.	Hassig, C. A., T. C. Fleischer, A. N. Billin, S. L. Schreiber, and D. E. Ayer. 1997. Histone deacetylase activity is required for full transcriptional repression by mSin3A. Cell 89:341-347[CrossRef][Medline].
19.	Horiuchi, J., N. Silverman, G. A. Marcus, and L. Guarente. 1995. ADA3, a putative transcriptional adaptor, consists of two separable domains and interacts with ADA2 and GCN5 in a trimeric complex. Mol. Cell. Biol. 15:1203-1209[Abstract].
20.	Hurlin, P. J., C. Queva, P. J. Koskinen, E. Steingrimsson, D. E. Ayer, N. G. Copeland, N. A. Jenkins, and R. N. Eisenman. 1995. Mad3 and Mad4: novel Max-interacting transcriptional repressors that suppress c-myc dependent transformation and are expressed during neural and epidermal differentiation. EMBO J. 14:223-232.
21.	Kato, G. J., J. Barrett, M. Villa-Garcia, and C. V. Dang. 1990. An amino-terminal c-Myc domain required for neoplastic transformation activates transcription. Mol. Cell. Biol. 10:5914-5920[Abstract/Free Full Text].
22.	Laherty, C. D., W. M. Yang, J. M. Sun, J. R. Davie, E. Seto, and R. N. Eisenman. 1997. Histone deacetylases associated with the mSin3 corepressor mediate Mad transcriptional repression. Cell 89:349-356[CrossRef][Medline].
23.	Lahoz, E. G., L. Xu, N. Schreiber-Agus, and R. A. DePinho. 1994. Suppression of Myc, but not E1a, transformation activity by Max-associated proteins, Mad and Mxil. Proc. Natl. Acad. Sci. USA 91:5503-5507[Abstract/Free Full Text].
24.	Luo, R. X., A. A. Postigo, and D. C. Dean. 1998. Rb interacts with histone deacetylase to repress transcription. Cell 92:463-473[CrossRef][Medline].
25.	MacGregor, D., L. H. Li, and E. B. Ziff. 1996. Dominant negative mutants of Myc inhibit cooperation of both Myc and adenovirus serotype-5 E1A with Ras. J. Cell. Physiol. 167:95-105[CrossRef][Medline].
26.	Magnaghi-Jaulin, L., R. Groisman, I. Naguibneva, P. Robin, S. Lorain, J. P. Le Villain, F. Troalen, D. Trouche, and A. Harel-Bellan. 1998. Retinoblastoma protein represses transcription by recruiting a histone deacetylase. Nature 391:601-605[CrossRef][Medline].
27.	Marcus, G., N. Silverman, S. Berger, J. Horiuchi, and L. Guarente. 1994. Functional similarity and physical association between GCN5 and ADA2: putative transcriptional adaptors. EMBO J. 13:4807-4815[Medline].
28.	Martinez, E., T. K. Kunda, J. Fu, and R. G. Roeder. 1998. A human SPT3-TAF_II31-GCN5-L acetylase complex distinct from transcription factor IID. J. Biol. Chem. 273:23781-23785[Abstract/Free Full Text].
29.	McMahon, S. B., H. A. VanBuskirk, K. A. Dugan, T. D. Copeland, and M. D. Cole. 1998. The novel ATM-related protein TRRAP is an essential cofactor for the c-Myc and E2F oncoproteins. Cell 94:363-374[CrossRef][Medline].
30.	Ogryzko, V. V., T. Kotani, X. Zhang, R. L. Schiltz, T. Howard, J. Quin, and Y. Nakatani. 1998. Histone-like TAFs within the PCAF histone acetylase complex. Cell 94:35-44[CrossRef][Medline].
31.	Ogryzko, V. V., R. L. Schiltz, V. Russanova, B. H. Howard, and Y. Nakatani. 1996. The transcriptional coactivators p300 and CBP are histone acetyltransferases. Cell 87:953-959[CrossRef][Medline].
32.	Peters, M. A., and E. J. Taparowsky. 1998. Target genes and cellular regulators of the Myc transcription complex. Crit. Rev. Eukaryot. Gene Expr. 8:277-296[Medline].
33.	Saleh, A., V. Lang, R. Cook, and C. J. Brandl. 1997. Identification of native complexes containing the yeast coactivator/repressor proteins NGG1/ADA3 and ADA2. J. Biol. Chem. 272:5571-5578[Abstract/Free Full Text].
34.	Saleh, A., D. Schieltz, N. Ting, S. B. McMahon, D. W. Litchfield, J. R. Yates III, S. P. Lees-Miller, M. D. Cole, and C. J. Brandl. 1998. Tra1p is a component of the yeast ADA/SPT transcriptional regulatory complexes. J. Biol. Chem. 273:26559-26570[Abstract/Free Full Text].
35.	Sarid, J., T. D. Halazonetis, W. Murphy, and P. Leder. 1987. Evolutionarily conserved regions of the human c-myc protein can be uncoupled from transforming activity. Proc. Natl. Acad. Sci. USA 84:170-173[Abstract/Free Full Text].
36.	Schreiber-Agus, N., L. Chin, K. Chen, R. Torres, G. Rao, P. Guida, A. I. Skoultchi, and R. A. DePinho. 1995. An amino-terminal domain of Mxi1 mediates anti-Myc oncogenic activity and interacts with a homolog of the yeast transcriptional repressor SIN3. Cell 80:777-786[CrossRef][Medline].
37.	Smith, E. R., J. M. Belote, R. L. Schiltz, X.-J. Yang, P. A. Moore, S. L. Berger, Y. Nakatani, and C. D. Allis. 1998. Cloning of Drosophila GCN5: conserved features among metazoan GCN5 family members. Nucleic Acids Res. 26:2948-2954[Abstract/Free Full Text].
38.	Smith, E. R., A. Eisen, W. Gu, M. Sattah, A. Pannuti, J. Zhou, R. G. Cook, J. C. Lucchesi, and C. D. Allis. 1998. ESA1 is a histone acetyltransferase that is essential for growth in yeast. Proc. Natl. Acad. Sci. USA 95:3561-3565[Abstract/Free Full Text].
39.	Spencer, T. E., G. Jenster, M. M. Burcin, C. D. Allis, J. Zhou, C. A. Mizzen, N. J. McKenna, S. A. Onate, S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1997. Steroid receptor coactivator-1 is a histone acetyltransferase. Nature 389:194-198[CrossRef][Medline].
40.	Stone, J., T. DeLange, G. Ramsay, E. Jakobovits, J. M. Bishop, H. Varmus, and W. Lee. 1987. Definition of regions in human c-myc that are involved in transformation and nuclear localization. Mol. Cell. Biol. 7:1697-1709[Abstract/Free Full Text].
41.	Struhl, K. 1998. Histone acetylation and transcriptional regulatory mechanisms. Genes Dev. 12:599-606[Free Full Text].
42.	Vassilev, A., J. Yamauchi, T. Kotani, C. Prives, M. L. Avantaggiati, J. Qin, and Y. Nakatani. 1998. The 400 kDa subunit of the PCAF histone acetylase complex belongs to the ATM superfamily. Mol. Cell 2:869-875[CrossRef][Medline].
43.	vom Baur, E., M. Harbers, S. J. Um, A. Benecke, P. Chambon, and R. Losson. 1998. The yeast Ada complex mediates the ligand-dependent activation function AF-2 of retinoid X and estrogen receptors. Genes Dev. 12:1278-1289[Abstract/Free Full Text].
44.	Wang, L., L. Liu, and S. L. Berger. 1998. Critical residues for histone acetylation by GCN5, functioning in Ada and SAGA complexes, are also required for transcriptional function in vivo. Genes Dev. 12:640-653[Abstract/Free Full Text].
45.	Wang, L., C. Mizzen, C. Ying, R. Candau, N. Barlev, J. Brownell, C. D. Allis, and S. L. Berger. 1997. Histone acetyltransferase activity is conserved between yeast and human GCN5 and is required for complementation of growth and transcriptional activation. Mol. Cell. Biol. 17:519-527[Abstract].
46.	Wieczorek, E., M. Brand, X. Jacq, and L. Tora. 1998. Function of TAF(II)-containing complex without TBP in transcription by RNA polymerase II. Nature 393:187-191[CrossRef][Medline].
46a.	Wood, M. A., S. B. McMahon, and M. D. Cole. An ATPase/helicase complex is an essential cofactor for oncogenic transformation by c-Myc. Mol. Cell, in press.
47.	Wu, S., A. Pena, A. Korcz, D. R. Soprano, and K. J. Soprano. 1996. Overexpression of Mxi1 inhibits the induction of the human ornithine decarboxylase gene by the Myc/Max protein complex. Oncogene 12:621-629[Medline].
48.	Yang, X.-J., V. V. Ogryzko, J. Nishikawa, B. H. Howard, and Y. Nakatani. 1996. A p300/CBP-associated factor that competes with the adenoviral oncoprotein E1A. Nature 382:319-324[CrossRef][Medline].
49.	Zawel, L., and D. Reinberg. 1995. Common themes in assembly and function of eukaryotic transcription complexes. Annu. Rev. Biochem. 64:533-561[CrossRef][Medline].
50.	Zervos, A., J. Gyuris, and R. Brent. 1993. Mxi1, a protein that specifically interacts with Max to bind Myc-Max recognition sites. Cell 72:223-232[CrossRef][Medline].
51.	Zhang, Y., R. Iratni, H. Erdjument-Bromage, P. Tempst, and D. Reinberg. 1997. Histone deacetylases and Sap18, a novel polypeptide, are components of a human Sin3 complex. Cell 89:357-364[CrossRef][Medline].