The Androgen Receptor Amino-Terminal Domain Plays a Key Role in p160 Coactivator-Stimulated Gene Transcription

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Molecular and Cellular Biology, September 1999, p. 6085-6097, Vol. 19, No. 9
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The Androgen Receptor Amino-Terminal Domain Plays a Key Role in p160 Coactivator-Stimulated Gene Transcription

Philippe Alen,¹^, Frank Claessens,¹ Guido Verhoeven,² Wilfried Rombauts,¹ and Ben Peeters¹^,^*

Division of Biochemistry¹ and Laboratory for Experimental Medicine and Endocrinology,² Faculty of Medicine, University of Leuven, B-3000 Leuven, Belgium

Received 31 March 1999/Returned for modification 5 May 1999/Accepted 11 May 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Steroid receptors are conditional transcription factors that, upon binding to their response elements, regulate the expressionof target genes via direct protein interactions with transcriptionalcoactivators. We have analyzed the functional interactions betweenthe androgen receptor (AR) and 160-kDa nuclear receptor coactivators.Upon overexpression in mammalian cells, these coactivators enhancethe transcriptional activity of both the amino-terminal domain(NTD) and the ligand-binding domain (LBD) of the AR. The coactivatoractivity for the LBD is strictly ligand-controlled and dependson the nature of the DNA-binding domain to which it is fused.We demonstrate that the NTD physically interacts with coactivatorsand with the LBD and that this interaction, like the functionalinteraction between the LBD and p160 coactivators, relies on theactivation function 2 (AF2) core domain. The mutation of a highlyconserved lysine residue in the predicted helix 3 of the LBD (K720A),however, blunts the functional interaction with coactivators butnot with the NTD. Moreover, this mutation does not affect thetranscriptional activity of the full-size AR. A mutation in theNTD of activation function AF1a (I182A/L183A), which dramaticallyimpairs the activity of the AR, has no effect on the intrinsictranscriptional activity of the NTD but interferes with the cooperationbetween the NTD and the LBD. Finally, p160 proteins in which thethree LXXLL motifs are mutated retain most of their coactivatoractivity for the full-size AR, although they are no longer functionalfor the isolated LBD. Together, these data suggest that in thenative AR the efficient recruitment of coactivators requires afunctional association of the NTD with the LBD and that the bindingof coactivators occurs primarily through theNTD.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Steroid receptors, including the androgen receptor (AR), belong to the superfamily of nuclear receptors (NRs) which generallyact as ligand-dependent transcription factors. In the absenceof ligand, they are maintained in an inactive state complexedto heat shock proteins and/or corepressors. Binding of the cognateligand results in the dissociation of the receptor from this inactivecomplex and its subsequent translocation to the nucleus, whereit binds, either as a homo- or a heterodimer, to specific responseelements in the promoter and/or enhancer regions of responsivegenes and up- or downregulates their transcription (37, 49,62). NRs share a common structural and functional organizationand generally harbor two transcription activation functions (AF):a constitutively active AF1, which is located in the highly variableNH₂-terminal domain (NTD) of the receptor, and a ligand-dependentAF2, which colocalizes with the more conserved COOH-terminal ligand-bindingdomain (LBD) (6). Whereas the molecular mechanisms by whichAF1 stimulates transcription are still largely unknown, our knowledgeof the functioning of AF2 has greatly increased in the past fewyears, most notably after the discovery of a new class of proteinscalled NR coactivators and after the crystal structures of apo-and holo-LBDs of several NRs became available (42, 51, 67,69). The LBD structurally consists of twelve $alpha$ -helices, themost COOH-terminal of which (helix 12[H12]) is projected awayfrom the hormone-binding pocket in the absence of ligand. Afterthe association of the LBD with an agonist, H12 "flips over" andcovers the hydrophobic ligand-binding cavity as a lid (47).Apart from keeping the ligand tightly bound as a "mouse in a trap",the swinging of H12 also has important structural consequencesand induces the formation of a new structural surface which caninteract with accessory proteins. A plethora of proteins havebeen identified which interact, mostly in a ligand-dependent way,with the LBDs of NRs and which can stimulate or repress AF2 activity(reviewed in references 23, 27, and 52). The best-characterizedsubgroup of receptor-interacting proteins is the family of 160-kDaNR coactivators, also called p160 proteins, comprising (i) steroidreceptor coactivator-1 (SRC-1) (29, 30, 45, 57), (ii)the human and rat transcription-intermediary factor 2 (TIF2) (34,64, 65) and its mouse orthologue glucocorticoid receptor (GR)-interactingprotein 1 (GRIP1) (21), and (iii) receptor-associated coactivator3 (RAC3) (35, 36), also known as ACTR (12), TRAM-1 (58),AIB (3), p/CIP (60), and SRC-3 (56). They interact withthe LBD via a centrally located NR-interacting region (NIR) containingthree highly conserved $alpha$ -helical LXXLL motifs, or NR boxes (19,29, 35, 36, 46, 50, 60, 65). One isoform of SRC-1(SRC-1a) contains a fourth NR box at its extreme carboxy terminus(29, 30), which is absent in another isoform called SRC-1e.Although this SRC-1a-specific NR box IV can interact with theLBDs of NRs (14, 19, 29, 59), the relevance of this interactionremains unestablished (29, 59). In addition, the carboxy-terminalend of SRC-1a harbors a repressive function that affects its coactivatoractivity for the estrogen receptor (ER) AF2 function (29).

Mutational analyses of the LBDs of a variety of NRs have revealed that, among others, a conserved lysine residue in H3 andthe AF2 core domain located in H12 are essential for the interactionof the receptors with p160 proteins and for transcriptional activity(12, 13, 17, 20, 58, 61). The X-ray structure of aternary complex of the peroxisome proliferator-activated receptor(PPAR) LBD with rosiglitazone and a fragment of SRC-1 comprisingtwo NR boxes (43) showed that this lysine and a conserved glutamatein H12 form a "change clamp" that forms hydrogen bonds with backboneamides of the LXXLL motifs, whereas the hydrophobic face of theLXXLL helix fits into a hydrophobic cavity. It was reported veryrecently that the ER AF1 domain may also function via the recruitmentof p160 proteins (66), but this interaction does not dependon the LXXLLmotifs.

Most of our knowledge of the action mechanism of NRs, and most notably of their AF2s, comes from studies with the retinoicacid and retinoid X receptors (RAR and RXR), the thyroid hormonereceptor (TR), and the ER. A striking difference between thesereceptors and the AR is that for the latter an intrinsic AF2 activityin the LBD has remained elusive (25, 40, 53), despite therelatively high degree of sequence similarity of its LBD withthat of other steroid receptors (67, 69). The AF1 function,on the other hand, has received more attention and was characterizedby several groups (11, 24, 26). The observation that differentactivation regions within the NTD are used in a full-length receptorand in a constitutively active mutant, devoid of the LBD, indicatesthat the activity of the NTD may be controlled by the LBD andraises the possibility of a functional interaction between thesedomains. Such an interaction could be demonstrated in classicalyeast and mammalian two-hybrid experiments (8, 15, 24,31) and was also observed for the ER (39). Moreover, evenin the absence of a heterologous transactivating domain, the humanAR (hAR) LBD and NTD can associate to form a transcriptionallyactive complex (8, 15). It is still unclear whether thisinteraction is direct or whether a third partner is involved whichwould act as a bridging factor. Possible candidates for such bridgingproteins are the p160 coactivators, since they were shown to enhancethe interaction between the NTD and the LBD of the AR and theER (24, 39).

In this paper, we describe the effects of p160 coactivators on the isolated AF1 and AF2 domains of the hAR. Furthermore, wehave analyzed the functional and physical interaction of theseAFs with each other and with the coactivators by using point-mutatedproteins. Our data suggest that the interaction between the hARNTD and LBD may be a prerequisite for the efficient recruitmentof coactivators to the native receptor and for its transcriptionalactivity, thus highlighting a novel role for the NTD in the functioningof theAR.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Materials. The hAR expression vector pSG5-hAR and the K720A mutant are described elsewhere (2). The other mutants were made by a PCR-basedmethod. The I898A/I899A mutation was generated with the oligonucleotides5'-GATGGCAGAGGCCGCCTCTGTGCAAGATC-3' and 5'-GATCTTGCACAGAGGCGGCCTCTGCCATC-3',in which the underlined sequences represent the mutated codons.To generate the AF1a mutation (I182A/L183A), the following oligonucleotideswere used: 5'-CCTTAAAGACGCCGCGAGCGAGGCC-3' and 5'-GGCCTCGCTCGCGGCGTCTTTAAGG-3'.Expression vectors for the hAR NTD (M1 to R538) and for DNA-bindingdomain (DBD)-LBD (L539 to Q919) were made by inserting PCR-generatedfragments encoding the corresponding regions in the BamHI siteof pSG5. Similarly, the DBD-LBD fragment of the rat GR (rGR) (P416to K777) was PCR amplified from pH6GR (a gift from H. Stunnenberg)and subcloned in the BamHI site of pSG5. The expression vectorfor the NTD-DBD was a kind gift from A. O. Brinkmann (25). Forthe expression of receptor domains fused to residues 1 to 147of the yeast transcription factor GAL4, PCR-generated fragmentsencoding either the NTD (M1 to R538) or the LBD (A628 to Q919)were inserted in the BamHI restriction site of pAB-Gal4 (4).The reporter plasmid pGal-50hIL6-luc (48), containing two GAL4-bindingsites in front of the minimal promoter of the human interleukin6 (hIL6) gene, was a kind gift of S. Plaisance. For the expressionof glutathione S-transferase (GST) fusion proteins, the plasmidpHIL was constructed by inserting two complementary oligonucleotidesencoding the vesicular stomatitis virus (VSV)-G epitope tag (NH₂-MYTDIEMNRLGKG-COOH)in the BamHI site of pCMV-GST (63). Next, the DNA fragmentsencoding the DBD-LBD regions of the murine ER (mER) and the hARwere isolated from the corresponding expression plasmids and insertedinto pHIL. The resulting vectors drive the expression of fusionproteins consisting of GST, the VSV-G tag, and the entire DBDand LBD of the respective receptors. To generate VP16 fusion proteinsfor use in mammalian double-hybrid experiments, a modified versionof the plasmid pSNATCH was used (10). A cDNA-fragment encodingthe residues 454 to 498 of the VP16 activating domain was insertedin pSNATCH, giving rise to pSNATCH-II, which thus directs theexpression of the residues 413 to 498 of the VP16 activating region.Finally, the hAR NTD was cloned in frame with the VP16 activatingdomain in the BglII site of pSNATCH-II. Expression vectors forTIF2 and for SRC-1, and derivatives thereof, were obtained fromH. Gronemeyer and M. G. Parker, respectively. All PCRs were performedwith the Pwo thermostable DNA polymerase (Boehringer, Mannheim,Germany). Restriction and modifying enzymes were obtained, eitherfrom Boehringer, Pharmacia (Uppsala, Sweden), or Life Technologies(Grand Island, N.Y.). The synthetic androgens R1881 (methyltrienolone)and mibolerone were supplied by Dupont-New England Nuclear (Boston,Mass.), and the synthetic glucocorticoid hormone triamcinoloneacetonide was from Sigma (St. Louis, Mo.). [³H]mibolerone (82.3 Ci/mmol) was purchased from Amersham (Buckinghamshire,UnitedKingdom).

Transfections. All transfections were performed in COS 7 cells or in CV-1 cells, obtained from the American Type Culture Collection (Rockville,Md.). One day prior to transfection, the cells were seeded in24-well culture plates in Dulbecco's modified eagle's medium (LifeTechnologies) containing 5% dextran-coated charcoal-stripped fetalbovine serum (DCC) at a density of 7.5 × 10⁴ per well. They were transfected, either by the calcium phosphatecoprecipitation method or with the Fugene 6 transfection reagent(Boehringer). After transfection, the cells were incubated for24 h with DCC-treated medium, either supplemented or not withhormones (1 nM). Finally, they were washed twice with phosphate-bufferedsaline (PBS) and lysed in 100 µl of passive lysis buffer (PromegaCorp., Madison, Wis.). The protein concentration was measuredwith the Coomassie protein assay reagent from Pierce (Rockford,Ill.). The luciferase and $beta$ -galactosidase activities were measuredon 10 µl of the extracts with the assay systems from Promega andClontech (Palo Alto, Calif.), respectively, and corrected forprotein content. The luciferase activity was corrected for transfectionefficiency by normalizing it against $beta$ -galactosidase activity.The total amount of DNA that was transfected depended on the transfectionmethod that was used, but the relative proportions were always10/1/10 for reporter-receptor-coactivator cotransfections. Theamount of pCMV- $beta$ -GAL was fixed at 50 ng per well. Where applicable,empty pSG5 vector was added to keep the total amount of transfectedDNA constant. The transfection results are always shown as themeasured luciferase activity, relative to a standard conditionas mentioned in the legends to the respective figures. The valuesshown are the means of at least three measurements ± the standarderror of the mean(SEM).

In vivo ligand binding and immunoblotting. Androgen binding was measured in transiently transfected COS 7 cells as follows: on day 1 the cells were transfected in 175-cm² tissue culture flasks with 10 µg of expression vector for eitherthe wild-type hAR or the K720A or I898A/I899A mutants by the calciumphosphate coprecipitation technique. The precipitate was lefton the cells for 16 h, after which they received a 15% glycerolshock for 2 min and were incubated in DCC-treated medium. On day3, they were trypsinized and seeded in 24-well plates at a densityof 10⁵ per well and were seeded in 60-mm-diameter dishes at a densityof 2.5 × 10⁵ per dish. On day 4, the cells in the 24-well plates were incubatedwith DCC-treated medium containing increasing concentrations of[³H]mibolerone, (0.1 to 100 nM), either in the absence or in thepresence of a 200-fold excess of unlabeled hormone to eliminatenonspecific binding. After 90 min at 37°C, the plates were puton melting ice and the cells were washed twice with ice-cold PBS.They were lysed in 100 µl of 0.1 N NaOH-1% Triton X-100, and theradioactivity was measured in a scintillation counter. K_d valueswere calculated by the Scatchard method. For Western blotting,the cells in the 60-mm-diameter dishes were lysed by two cyclesof freezing in liquid N₂ and thawing at room temperature in 20mM Tris (pH 7.8)-300 mM NaCl-1 mM EDTA-0.1% Nonidet P-40 and solubleextracts were prepared by centrifugation. Ten microliters of eachextract was separated by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) in an 8% gel and blotted onto polyvinylidenedifluoride membranes. The membranes were probed with a polyclonalantiserum against the NH₂ terminus of the hAR (38), and immunoreactiveproteins were visualized with the ECL system(Amersham).

GST pull down. For GST pull-down experiments, COS cells in 9-cm-diameter plates were cotransfected with expression vectors for the respectiveGST fusion proteins (described above) and FLAG-tagged SRC-1e orthe NTD by the calcium phosphate coprecipitation procedure. Aftertransfection, the cells were incubated for 24 h with medium withor without 100 nM of the appropriate hormone. The cells were washedtwice with ice-cold PBS, and extracts were prepared by two cyclesof freezing in liquid nitrogen and thawing on ice in 50 µl ofNENT₃₀₀-Mo (20 mM TRIS [pH 6.8], 300 mM NaCl, 1 mM EDTA, 0.1%Nonidet P-40, 25% glycerol, 20 mM Na molybdate), followed by centrifugationto pellet insoluble material. The extracts were diluted with 150µl of NENT₀-Mo (like NENT₃₀₀-Mo but lacking NaCl) and loaded ontoglutathione-Sepharose beads (Pharmacia). The GST fusion proteinswere then allowed to bind to the matrix for 16 h at 4°C on a rotatingwheel. The beads were washed extensively with NENT₁₀₀-Mo, andbound proteins were eluted by boiling the matrix in SDS-PAGE samplebuffer, subjected to SDS-PAGE, and finally blotted onto polyvinylidenedifluoride membranes. Hormone (100 nM) was included in all buffers,where applicable. To visualize FLAG-SRC-1e, Western blots wereprobed with an M2 anti-FLAG antibody (Stratagene, La Jolla, Calif.),and to detect the hAR NTD, a polyclonal antiserum recognizingthe first 20 residues of the hAR was used (38). To ensure adequateexpression of all GST fusion proteins, aliquots of the COS extractswere immunoblotted with a monoclonal anti-VSV-G antibody(Sigma).

	RESULTS

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Both the hAR AF1- and AF2-containing domains, when expressed separately, can be stimulated by p160 coactivators. The observation that, contrary to many other NRs, the hAR LBD has no detectable intrinsic AF2 activity in mammalian cells(26, 40, 53) prompted us to analyze the effect of p160 coactivatorson the transcriptional activity of this receptor. Cotransfectionexperiments in COS cells, using the androgen-responsive MMTV-lucvector as a reporter, reveal that p160 proteins stimulate theligand-dependent transcriptional activity of the hAR (Fig. 1A).In the absence of ectopically expressed coactivator, the luciferaseactivity is stimulated approximately 10-fold in response to 1nM synthetic androgen R1881 (Fig. 1, bar 1), whereas cotransfectionof TIF2, SRC-1a, or SRC-1e results in a further 4- to 6-fold increaseof transcription (bars 2 to 4). To ensure that the presence inCOS cells of the large T antigen and the concomitant high expressionlevels of proteins encoded by pSG5-based plasmids did not influencethe observed effects, we also performed the experiment in CV-1cells. As shown in Fig. 1B, similar results were obtained underthese conditions. It should be noted that the absolute levelsof luciferase activity measured in CV-1 cells are on average 5to 10 times lower than those measured in COS cells under the sameexperimental conditions.

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FIG. 1. p160 coactivators stimulate the transcriptional activity of the full-size hAR. COS 7 cells (A) and CV-1 cells (B) were cotransfected with pMMTV-luc (500 ng) and pSG5-hAR (50 ng), along with 500 ng of either empty pSG5 (bar 1) or pSG5-TIF2, pSG5-SRC-1a, or pSG5-SRC-1e (bar 2 to 4). The cells were incubated with DCC-treated medium, either supplemented (solid bars) or not (open bars) with 1 nM R1881 24 h before being harvested. The luciferase activities were corrected for transfection efficiency by using the $beta$ -galactosidase activities. The data are presented as relative activities (± SEM). The luciferase activity measured in the presence of ligand but without cotransfected coactivator was arbitrarily set to 100, and test values were calculated accordingly.

Originally, p160 coactivators were thought to stimulate only the ligand-dependent AF2 transcription activation function ofNRs. However, it has been reported that SRC-1 can also interact,in a ligand-independent way, with NRs mutated in the AF2 region(28), and recent data indicate that p160 coactivators may alsostimulate AF1 and promote the functional interaction between thetwo AFs (24, 46, 66). To determine the effect of these coactivatorson either AF of the hAR, COS cells or CV-1 cells were cotransfectedas above, except that expression vectors encoding either the NTDand the DBD (NTD-DBD) or the DBD and the LBD (DBD-LBD) (Fig. 2A)were used instead of a plasmid encoding the entire receptor. Consistentwith previously reported results (26), the NTD has intrinsictranscription activation properties (AF1) (Fig. 2B, compare bars2 and 1). Coexpression of TIF2 or SRC-1a results in only a slightincrease of AF1 activity (Fig. 2B, compare bars 3 and 4 to bars2), whereas coexpression of SRC-1e results in a 15-fold and a12-fold induction of transcription (bar 5 versus bar 2) in COScells and in CV-1 cells, respectively. The effect of the p160coactivators on the transcriptional activity of the LBD was analyzedin a similar way. The DBD-LBD construct has no intrinsic ligand-dependenttranscription activation properties (Fig. 2C, bars 1), but coexpressionof either TIF2 or SRC-1e results in a strong induction of transcription(compare bars 2 and 4 to bars 1), as does coexpression of thehAR NTD (bars 5). SRC-1a, on the other hand, is a less potentcoactivator for the hAR DBD-LBD construct (bars 3), especiallyunder the conditions of high expression levels in COS cells (Fig.2C, upper panel). Similar to the effects on the full-size receptor(Fig. 1), the induction of transcriptional activity of the DBD-LBDfragment by overexpression of p160 proteins is strictly liganddependent. These experiments were also performed in COS cellswith constructs encoding the DBD of the yeast transcription factorGAL4 fused to either the hAR NTD or the hAR LBD (Fig. 2A) anda luciferase reporter gene, driven by five copies of a GAL4 DNA-bindingsite in front of a TATA box [(G4)₅-tata-luc]. The results obtainedwith the G4-NTD construct (Fig. 2D) are very similar to thoseobtained with the NTD-DBD construct and the MMTV-luc reporterdescribed in Fig. 2B. Whereas TIF2 and SRC-1a influence the activityof G4-NTD only weakly (Fig. 2B, compare bars 3 and 4 with bar2), SRC-1e clearly coactivates this construct to a much greaterextent (bar 5). Although the absolute levels of transcriptionstimulation of G4-NTD are somewhat lower than those obtained forthe NTD-DBD construct (4-fold versus 15-fold for SRC-1e), theeffects of either p160 protein are comparable under both conditions.Surprisingly, this is not the case when DBD-LBD and G4-LBD arecompared. Whereas TIF2 and SRC-1e strongly stimulate the activityof DBD-LBD (Fig. 2C), they have only minor effects on G4-LBD (Fig.2E; compare bars 3 to 5 with bar 2). hAR-NTD, on the other hand,does strongly stimulate the transcriptional activity of G4-LBD(to 23-fold [bar 6]).

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FIG. 2. The hAR AF1 and AF2 functions are both stimulated by p160 coactivators. (A) Schematic representation of the hAR and the constructs used in this study. Depicted are the NTD, the centrally located DBD, the hinge region (hatched box), and the C-terminal LBD of the hAR, and the DBD of the yeast transcription factor GAL4 (G4). The numbers refer to amino acid positions. **, position of the residues mutated in the AF1a mutant (I182A/L183A); $diamond$ , position of the H3 mutant (K720A); $triangle$ $triangle$ , position of the AF2 mutant (I898A/I899A). (B) COS cells (upper graph) and CV-1 cells (lower graph) were transfected with pMMTV-luc (250 ng) without (bars 1) or with (bars 2 to 5) an expression vector encoding NTD-DBD (125 ng) and with either empty pSG5 (bars 1 and 2) or pSG5-TIF2, pSG5-SRC-1a, or pSG5-SRC-1e (900 ng). After 24 h, the cells were harvested and luciferase and $beta$ -galactosidase activities were measured as described in Materials and Methods. The activity of NTD-DBD in the absence of exogenously added coactivator was given the value 100. All other activities were calculated accordingly. (C) COS cells (upper graph) and CV-1 cells (lower graph) were cotransfected with pMMTV-luc (250 ng), pSG5-DBD/LBD (25 ng), and either empty pSG5 (bar 1) or pSG5-TIF2, pSG5-SRC-1a, or pSG5-SRC-1e (250 ng) (bars 2 to 5) and incubated for 24 h in DCC-treated medium, either supplemented (solid bars) or not (open bars) with 1 nM R1881. They were harvested and processed as described in Materials and Methods. (D) COS 7 cells were transfected with the p(G4)₅-tata-luc reporter (250 ng) without (bar 1) or with (bars 2 to 5) an expression vector for G4-NTD (25 ng) and with either empty pSG5 (bars 1 and 2) or pSG5-TIF2, pSG5-SRC-1a, or pSG5-SRC-1e (bars 3 to 5; 250 ng) and treated as described for panel B. (E) COS 7 cells were transfected as for Fig. 2C, except that the p(G4)₅-tata-luc reporter vector was used and pSG5-DBD/LBD was replaced by an expression vector encoding G4-LBD. The cells were treated with 1 nM R1881 as indicated. The luciferase activity measured in the presence of R1881 but without ectopically expressed coactivator (bar 2) was set to 100, and test values were calculated accordingly. The error bars indicate the SEM.

A recent report suggested that the coactivator activity of TIF2 for the hAR AF2 function might be promoter dependent (8).To verify that the differences we observed between DBD-LBD andMMTV-luc on the one hand (Fig. 2C) and G4-LBD and (G4)₅-tata-lucon the other hand (Fig. 2E) are not merely the result of usinga complex MMTV-luc reporter versus a minimal (G4)₅-tata-luc reporter,we extended the experiments with G4-LBD to two other GAL4-drivenreporter constructs with more complex promoters: (G4)₅-TK-lucand Gal-50hIL6-luc containing 5 and 2 GAL4 DNA-binding sites,respectively, in front of the thymidine kinase (TK) promoter orthe minimal promoter of the human interleukin 6 gene (48). Asshown in Fig. 3, irrespective of the reporter used, coexpressionof the NTD always results in a potent activation of the transcriptionalactivity of G4-LBD, whereas coexpression of TIF2 results in onlya very poor stimulation of transcription.

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FIG. 3. hAR NTD efficiently stimulates the transcriptional activity of G4-LBD, independent of the promoter context. COS 7 cells were cotransfected with either p(G4)₅-tata-luc (left graph), p(G4)₅-TK-luc (center graph), or pGal-50hI16-luc (right graph), along with pG4-LBD and either empty pSG5 (bars 1, 2, 5, 6, 9, and 10), pSG5-TIF2 (bars 3, 7, and 11), or pSG5-NTD (bars 4, 8, and 12), as for Fig. 2E. The cells were incubated with DCC-treated medium, either supplemented (+) or not ( $-$ ) with 1 nM R1881 for 24 h and subsequently processed as described in Materials and Methods. In each case, the luciferase activity measured in the presence of hormone but in the absence of exogenously added coactivator was arbitrarily set to 100, and the values for the other conditions were calculated accordingly. The error bars indicate the SEM.

The hAR NTD physically interacts with SRC-1e and with the hAR LBD in COS cells. To examine whether the stimulatory effects we observed upon cotransfection of p160 proteins with either the isolated NTD orLBD can be correlated with direct protein-protein interactions,we performed GST pull-down experiments from transfected-cell extracts.Therefore, vectors were constructed directing the expression ofthe hAR NTD or of the DBD-LBD of the hAR and the mER, respectively,fused in frame to GST and the VSV-G tag, which were then cotransfectedin COS cells with a FLAG-tagged SRC-1e expression vector. Proteincomplexes associated with the GST fusion proteins were precipitatedfrom whole-cell extracts with a glutathione-Sepharose affinitymatrix and subsequently immunoblotted with anti-FLAG antibody.As shown in Fig. 4A, SRC-1e can be precipitated specifically byGST-NTD, indicating that the hAR NTD physically interacts withSRC-1e in COS cells. Using this technique, however, we were unableto demonstrate a strong physical interaction between the hAR DBD-LBDand SRC-1e, either in the absence or in the presence of ligand(Fig. 4B, lanes 2 and 3). Nevertheless, under the same experimentalconditions we saw a good ligand-dependent interaction of SRC-1ewith the GST-DBD-LBD construct of the mER (lanes 4 and 5). Aliquotsof the extracts were immunoblotted and probed with anti-VSV-Gantibody to ensure adequate expression of the mER and hAR GST-DBD-LBDfusion proteins (data not shown). This result indicates that thehAR LBD has very low intrinsic affinity for p160 proteins. However,in yeast and mammalian double-hybrid experiments we saw a ligand-dependentinteraction between the AR LBD and TIF2.5, a fragment of TIF2harboring the three NR box motifs (65). Compared to the interactionobserved with the LBD of a panel of NRs with a strong intrinsicAF2 activity, however, the AR LBD-TIF2.5 interaction is much weaker(our unpublished results).

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FIG. 4. hAR NTD physically interacts with SRC-1e and with the hAR LBD in COS cells. (A) COS cells were transfected with expression vectors for either GST alone or a fusion protein of GST with the hAR NTD, along with an expression vector for FLAG-tagged SRC-1e. After 24 h of incubation at 37°C, extracts were prepared and protein complexes bound to GST or GST-NTD were precipitated with glutathione Sepharose beads, immunoblotted, and stained with monoclonal anti-FLAG antibody. (B) COS cells were transfected and treated as described for panel A, except that GST fusion proteins of the DBD-LBD regions of the hAR and the mER were used. The cells were treated without hormone (lanes 1, 2, and 4) or with 100 nM of either R1881 (lane 3) or estradiol (lane 5) 24 h prior to the preparation of protein extracts and GST pull down. (C) COS cells were transfected and treated as for panel B, except that an expression vector for the hAR NTD was used instead of FLAG-tagged SRC-1e. The immunoblots were probed with a polyclonal anti-AR antiserum. +, present; $-$ , absent.

The GST pull-down experiment was also performed with an expression vector for the hAR NTD instead of FLAG-tagged SRC-1e, andthe precipitated complexes were immunoblotted with a polyclonalantiserum against the hAR NTD (38). The hAR NTD can be precipitatedspecifically and in a ligand-dependent way with the GST-DBD-LBDfusion protein (Fig. 4C, lanes 2 and 3), pointing to a physicalinteraction between the NTD and the LBD of thehAR.

The hAR NTD stimulates the transcription activation function of the hAR LBD more efficiently than that of the rGR LBD. The observation that the hAR NTD efficiently stimulates the hAR AF2 function raises the question whether this is a receptor-specificeffect or whether the AR NTD can also activate the AF2 functionof another steroid receptor, such as the rGR. To test this, aconstruct was made encoding the entire DBD and LBD of the rGR[here called DBD-LBD(GR)], similar to the DBD-LBD construct ofthe hAR [here called DBD-LBD(AR)]. Both constructs were transfectedin COS cells, along with the MMTV-luc reporter plasmid and withor without an expression vector for the hAR NTD. As shown in Fig.5 and consistent with the results described above, the hAR AF2activity is efficiently activated upon coexpression of the hARNTD (Fig. 5, compare bar 3 to bar 2). Contrary to DBD-LBD(AR),however, DBD-LBD(GR) has a good intrinsic ligand-dependent AF2function (Fig. 5, compare bars 5 and 4), and the addition of thesynthetic glucocorticoid hormone triamcinolone acetonide resultsin a 35-fold increase of reporter gene expression. Cotransfectionof the hAR NTD, however, stimulates the DBD-LBD(AR) 59-fold (Fig.5, bar 3 versus bar 2), whereas it has less pronounced effects(3-fold induction) on the AF2 activity of DBD-LBD(GR). Alternatively,the rGR NTD does not stimulate the transcriptional activity ofthe hAR LBD, nor does it strongly affect the rGR AF2 activity(data not shown). Note that the total transcriptional activitiesof either DBD-LBD construct in the presence of the hAR NTD arecomparable for the hAR and the rGR (Fig. 5, compare bars 3 and6).

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FIG. 5. Coexpression of the hAR NTD strongly stimulates the transcriptional activity of the hAR LBD but has only weak effects on the rGR AF2 function. COS 7 cells were transfected with 250 ng of pMMTV-luc, along with 25 ng of either pSG5-DBD/LBD(AR) or pSG5-DBD/LBD(GR) and 250 ng of either empty pSG5 (bar 1, 2, 4, and 5) or pSG5-NTD (bar 3 and 6), and treated for 24 h without hormone (bar 1 and 4), with 1 nM R1881 (bars 2 and 3), or with 1 nM triamcinolone acetonide (TA) (bars 5 and 6). Luciferase and $beta$ -galactosidase activities were measured as described in Materials and Methods. The luciferase activity measured with DBD-LBD(AR) in the presence of R1881 and in the absence of NTD (bar 2) was arbitrarily set to 100. The activities of all other conditions were calculated relative to this standard. The error bars indicate the SEM.

Effect of mutations in H3 and H12 of the LBD. The interaction between the p160 coactivators and nuclear receptors has been reported to occur primarily through residuesin H3, -4, -5, and -12 of the LBD (17, 20, 42). We haveexchanged a highly conserved lysine residue in H3 (K720) and twobulky hydrophobic residues in H12 (I898 and I899) of the hAR LBDfor alanines, both of which dramatically impair the transcriptionactivation function of the mER (13, 20). The mutants are efficientlyexpressed, as could be judged from Western blots of extracts oftransfected COS cells (data not shown). Their ability to bindligand was analyzed in a whole-cell ligand-binding assay. Thefollowing K_d values were calculated for the synthetic hormonemibolerone (mean ± SEM): 2.53 nM (±0.15) for the native receptorand 4.08 nM (±0.31) and 3.13 nM (±0.38) for the K720A and theI898A/I899A mutants, respectively. Thus, these mutations do notsubstantially influence ligand binding and probably do not alterthe overall structure of thereceptor.

Next, the effects of these amino acid changes on the transcriptional activity of the hAR were examined. In the absence ofexogenous TIF2, the mutant K720A can be induced as well as thewild-type receptor by 1 nM R1881 (Fig. 6A, compare bars 5 and6 to bars 1 and 2), whereas the mutant I898A/I899A is transcriptionallyinactive (bars 9 and 10). All three receptors, however (the wild-typeprotein as well as both mutants), can be stimulated by coexpressingTIF2. Compared to control conditions (without ectopic expressionof TIF2), the unmutated receptor and the K720A mutant are stimulated10- and 8-fold, respectively, upon cotransfection of TIF2 (Fig.6A, compare bar 4 to bar 2 and bar 8 to bar 6). Although the absolutelevel of luciferase activity measured with the I898A/I899A mutantin the presence of TIF2 and R1881 (Fig. 6A, bar 12) is much lower,coexpression of TIF2 still enhances the activity of the I898A/I899Amutant (compare bar 12 to bar 10), possibly reflecting a coactivatoractivity of TIF2 on the NTD. This hypothesis is further supportedby the observation that SRC-1e, which is a better coactivatorfor the NTD, stimulates the I898A/I899A mutant to a greater extentthan TIF2 (data not shown).

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FIG. 6. The effect of the K720A and I898A/I899A mutations on the transcriptional activities of the native hAR and on the DBD-LBD construct. (A) COS 7 cells were cotransfected with 250 ng of pMMTV-luc and 25 ng of expression vector for either the full-size wild-type hAR, the K720A mutant, or the I898A/I899A mutant, along with 250 ng of either empty pSG5 (bars 1, 2, 5, 6, 9, and 10) or pSG5-TIF2 (bars 3, 4, 7, 8, 11, and 12) and incubated for 24 h with DCC-treated medium without (open bars) or with (solid bars) 1 nM R1881. The measured luciferase activities were corrected for protein content and $beta$ -galactosidase activity and are expressed as relative values, with the activity of the native receptor in the presence of R1881 taken as 100. (B) COS 7 cells were transfected as described for panel A, but instead of expression vectors for full-size receptors, 25 ng of the plasmids encoding the DBD-LBD fragments of either the wild-type receptor, the K720A or the I898A/I899A mutants were used, along with 250 ng of either empty pSG5 (bars 1, 2, 5, 6, 9, and 10), pSG5-TIF2 (bars 3, 7, and 11) or pSG5-NTD (bars 4, 8, and 12). The cells were either left untreated (bars 1, 5, and 6) or treated with 1 nM R1881 (bars 2 to 4, 6 to 8, and 10 to 12) for 24 h before being harvested. The luciferase activity measured for the wild-type DBD-LBD construct in the presence of hormone was taken as 100, and test values were calculated. (C) GST pull-down experiments were performed as described in Materials and Methods and in the legend to Fig. 4. The immunoblots were probed with an anti-AR antiserum. +, present; $-$ , absent. The error bars indicate the SEM.

To eliminate such effects and to analyze the consequences of the above-mentioned mutations solely on the AF2 function, DBD-LBDconstructs were made carrying the K720A and the I898A/I899A mutations.The K720A mutant can be activated by cotransfection of TIF2 (Fig.6B, compare bar 7 to bar 6), although clearly less efficientlythan the unmutated DBD-LBD (bar 7 versus bar 3). Mutation of thetwo isoleucines in H12 (I898A/I899A) has even more pronouncedeffects, and cotransfection of TIF2 results in a maximal twofoldstimulation of transcription (Fig. 6B, bar 11 versus bar 10).The effects of these mutations on the stimulation of AF2 by thehAR NTD were also studied. As shown in Fig. 6B, the K720A mutationdoes not affect stimulation by the NTD (Fig. 6B, compare bar 8to bar 4), whereas I898A/I899A does (compare bar 12 to bars 4and 8). In keeping with this are the results of GST pull-downexperiments (Fig. 6C). The hAR NTD can be precipitated from COScell extracts, in a ligand-dependent way, by GST fusion proteinsof the wild-type and the K720A mutated DBD-LBD (Fig. 6C, lanes1 to 5) but not by the I898A/I899A mutant (lanes 6 and7).

Mutation of the LXXLL motifs in p160 proteins affects their coactivator properties for hAR LBD but not for hAR NTD. In vitro and in vivo binding studies with several p160 family members have identified a centrally located NIR containing threehighly conserved LXXLL motifs, which are sufficient for interactionwith the NR AF2 domain (19, 29, 46, 60, 65). Our observationthat the hAR AF1 domain, but also a full-size receptor in whichthe AF2 function is mutated, can be stimulated by 160-kDa coactivatorsprompted us to look at the effect of the mutation of the LXXLLmotifs on the coactivator properties for the full-size hAR, aswell as for the isolated AF1 and AF2functions.

Both native TIF2 and a molecule in which the three LXXLL motifs are mutated (M123) act as efficient coactivators for the full-lengthhAR with MMTV-luc as a reporter (Fig. 7, left graph), althoughthe activity of the M123 mutant is somewhat (~30%) lower thanthat of wild-type TIF2 (compare bars 2 and 3 to bar 1). The sameexperiment was performed with the DBD-LBD construct (Fig. 7, centergraph). As expected, mutation of the three LXXLL motifs resultsin a complete loss of coactivator activity of TIF2 for the isolatedLBD (compare bars 5 and 6 to bar 4). AF1, on the other hand, canbe stimulated by both native and mutated TIF2 (Fig. 7, right graph).No significant differences were detected between the wild-typeand the M123 forms with respect to their ability to stimulatethe transcriptional activity of the NTD-DBD construct (comparebars 8 and 9 to bar 7).

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FIG. 7. The effect of mutation of the three LXXLL motifs in TIF2 on the transcriptional activity of the hAR. COS-7 cells were transfected with 250 ng of pMMTV-luc reporter and 25 ng of pSG5-hAR (left graph), 25 ng of pSG5-DBD/LBD (center graph), or 125 ng of NTD-DBD expression vector (right graph), along with either 250 ng (bars 1 and 4) or 900 ng (bar 7) of empty pSG5, 250 ng (bars 2 and 5) or 900 ng (bar 8) of pSG5-TIF2(WT), or 250 ng (bars 3 and 6) or 900 ng (bar 9) of pSG5-TIF2(M123). The cells transfected with NTD-DBD (right graph) were incubated for 24 h in DCC-treated medium, and those transfected with the native hAR or DBD-LBD (left and center graphs) received DCC-treated medium supplemented with 1 nM R1881 (solid bars) or vehicle (ethanol) alone (open bars). The luciferase activities were corrected for transfection efficiency by using the $beta$ -galactosidase activities. +, present; $-$ , absent. The error bars indicate the SEM.

Since SRC-1e has more pronounced effects on the activity of the hAR NTD (Fig. 2B), we also analyzed the effects of comparablemutations in SRC-1e and found that they are identical to the effectsdescribed here for TIF2 and TIF2(M123) (data notshown).

Mutation of AF1a blunts the functional interaction between the hAR NTD and LBD. Chamberlain et al. (11) reported that the mutation of an isoleucine and a leucine in the NTD of the rAR, located in a regionthey termed AF1a, dramatically impairs the transcriptional activityof thereceptor.

We mutated these residues to alanines (I182A/L183A) and looked at the effect of this point mutation on the transcriptionalactivity of the native receptor, both in the absence and in thepresence of cotransfected TIF2. Whereas transcription is induced10-fold by the addition of 1 nM R1881 to the wild-type receptor(Fig. 8A, bar 1), the I182A/L183A mutant can only be induced 2-fold(bar 3). Coexpression of TIF2, however, results in an efficient(~7-fold) stimulation of the ligand-dependent transcriptionalactivity of both receptors (bars 2 and 4 versus bars 1 and 3),possibly reflecting the stimulatory effect of p160 coactivatorson the intact AF1 and/or AF2 function.

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FIG. 8. Effect of mutation of the AF1a function on the functional NTD-LBD interaction. (A) COS 7 cells were cotransfected with 250 ng of pMMTV-luc and 25 ng of expression vector for the wild-type hAR or the I182A/L183A mutant, along with 250 ng of either empty pSG5 (bars 1 and 3) or pSG5-TIF2 (bars 2 and 4) and incubated with DCC-treated medium, supplemented with vehicle alone (ethanol) (open bars) or 1 nM R1881 (solid bars). The measured luciferase activities were corrected for $beta$ -galactosidase activity and are expressed as relative values, with the activity of the wild-type receptor in the presence of hormone but without coexpression of TIF2 set to 100. (B) COS cells were transfected with pMMTV-luc (250 ng), expression vectors for either the wild-type (bars 1 and 3) or the I182A/L183A mutated (bars 2 and 4) NTD-DBD constructs and either empty pSG5 (bars 1 and 2) or pSG5-SRC-1e (bars 3 and 4). Extracts were prepared, and luciferase activities and $beta$ -galactosidase activities were measured as described in Materials and Methods. (C) COS 7 cells were transfected with 250 ng of pMMTV-luc and 25 ng of expression plasmid for the wild-type DBD-LBD fragment, along with 250 ng of either empty pSG5 (bars 1 and 2) or expression vector for the wild-type hAR NTD (bar 3) or the NTD carrying the I182A/L183A mutation (bar 4). The cells were treated for 24 h without (bar 1) or with (bars 2 to 4) 1 nM R1881. The luciferase activities are presented relative to the activity measured in the presence of hormone but without cotransfected NTD. (D) GST pull-down experiments were carried out as for Fig. 4C with either GST alone or a GST-DBD-LBD fusion protein and the wild-type (lanes 1 to 3) or I182A/L183A mutated (lane 4) hAR NTD. (E) COS 7 cells were transfected as for panel C, except that plasmids directing the expression of the NTD fused to the VP16 activating domain were used. The luciferase activity measured in the presence of ligand but in the absence of VP16 fusion protein was taken as 100. Test values were calculated accordingly. +, present; $-$ , absent. The error bars indicate the SEM.

To investigate whether the effect of the AF1a mutation might be due to an impaired intrinsic transcription activation functionof the hAR NTD or to a loss of stimulation of AF1 by p160 proteins,transfections were performed with NTD-DBD constructs, either carryingor not carrying the I182A/L183A mutation, with or without cotransfectionof SRC-1e. The mutated NTD-DBD construct has intrinsic transcriptionactivation properties comparable to those of a wild-type construct(Fig. 8B, compare bars 2 and 1). Moreover, both constructs arestimulated equally well by coexpression of SRC-1e, indicatingthat these hydrophobic residues are probably not involved in theinteraction of the hAR NTD with p160coactivators.

Finally, the effect of the AF1a mutation on the functional interaction of the hAR NTD with the LBD was studied (Fig. 8C).Whereas the wild-type NTD efficiently stimulates the hAR AF2 function(compare bar 3 to bar 2), this effect is markedly reduced by themutation of AF1a (bar 4). The ability of the mutated NTD to physicallyinteract with the LBD was analyzed in the GST pull-down assayin COS extracts (Fig. 8D). In the presence of androgen, the wild-typehAR NTD interacts with the GST-DBD-LBD fusion protein (lanes 1to 3) whereas the NTD carrying the I182A/L183A mutations doesnot (lane 4). Similar conclusions can be drawn from mammaliandouble-hybrid experiments (Fig. 8E). Whereas the hAR LBD efficientlyinteracts with a fusion protein of the unmutated hAR NTD withthe VP16 acidic transactivating domain (bar 4), this interactionis severely impaired by the mutation of AF1a (bar 5 versus bar4).

The hAR NTD enhances the coactivator properties of TIF2 for the hAR LBD. Finally, we analyzed the effect on the transcriptional activity of the LBD of the simultaneous expression of the NTD and p160proteins. As shown in Fig. 9A, both in COS cells (left graph)and in CV-1 cells (right graph) the NTD and TIF2 or SRC-1e cooperativelystimulate the transcriptional activity of the hAR LBD. This effectis most pronounced in COS cells. Whereas, under these conditions,cotransfection of the DBD-LBD construct with either the NTD orp160 protein alone results in a ~10-fold induction of transcription(compare bars 3, 5, and 6 with bar 2), the simultaneous expressionof the NTD and 160-kDa coactivators results in an almost-100-foldinduction of transcription (compare bars 7 and 9 with bar 2).This effect relies on an intact AF1a region, since cotransfectionof the p160 coactivators with the I182A/L183A mutated NTD doesnot result in cooperativity (bars 8 and 10).

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FIG. 9. hAR NTD and TIF2 cooperatively stimulate the transcriptional activity of the hAR LBD. (A) COS-7 cells (left graph) or CV-1 cells (right graph) were cotransfected with 250 ng of pMMTV-luc, 25 ng of expression vector for the DBD-LBD construct, and 250 ng of expression vector for either the wild-type or I182A/L183A mutated NTD, for TIF2, or for SRC-1e as indicated. Under the conditions where only one cofactor was transfected (bars 1 to 6), empty pSG5 plasmid was added to keep the total amount of transfected DNA constant. The cells were incubated for 24 h without (bars 1) or with (bars 2 to 10) 1 nM R1881 before harvesting and measurement of luciferase and $beta$ -galactosidase activities. The luciferase activity measured in the presence of hormone, but without cotransfected NTD or coactivator (bars 2), was set to 100, and test values were calculated accordingly. (B) COS-7 cells (left graph) or CV-1 cells (right graph) were cotransfected with 250 ng of pMMTV-luc, 25 ng of expression vector for the DBD-LBD construct, and 250 ng of expression vector for the hAR NTD, TIF2(WT), or TIF2(M123), as indicated. For bars 1 to 4 and bars 6, empty pSG5 was added to keep the total amount of transfected DNA constant. The cells were further processed as described for panel A. +, present; $-$ , absent. The error bars indicate the SEM.

To analyze the importance of the three NR boxes in TIF2 for this cooperative stimulation of the transcriptional activity ofthe LBD, the same type of experiment was performed with the wild-typeNTD and with the wild-type or mutated TIF2. As shown in Fig. 9B,both in COS cells (left graph) and in CV-1 cells (right graph),cotransfection of the NTD with TIF2(M123) results in a markedincrease of the transcriptional activity of the LBD, comparedto conditions where either of these two components is transfectedalone (compare bars 7 to bars 3 and 6). Although the absolutereporter activity measured with the combination of the NTD andTIF2(M123) is lower than that measured with the combination ofthe NTD and wild-type TIF2 (Fig. 9B, compare bars 7 to bars 5),cotransfection of the NTD still reveals coactivator propertiesin the mutated TIF2. Note that the results of the cotransfectionof the NTD and the LBD with either wild-type or mutated TIF2 (bars5 and 7) are comparable to the effects seen after cotransfectionof the full-size hAR with TIF2 or TIF2(M123) (Fig. 7).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Upon cotransfection in COS or in CV-1 cells, 160-kDa NR coactivators stimulate the ligand-dependent transcriptional activityof the hAR. The currently accepted model to explain these effectsproposes that ligand binding induces conformational changes inthe LBD, resulting in a novel molecular surface that interactswith the coactivators (42, 61). These coactivators, like thereceptors themselves, interact with basal transcription factorsand serve to bring the transcription preinitiation complex andRNA polymerase II to the promoter (7, 57). Furthermore, thecoactivators have intrinsic histone-acetylase (HAT) activity (12,55), and interact with yet other HATs, such as CREB-bindingprotein (CBP) (5, 44) and p300/CBP-associated factor (p/CAF)(71), which in turn also bind to the receptors (1, 9,18). Following the acetylation of lysine residues in the tailsof core histones, the tight chromatin structure is relaxed andthe transcription apparatus can gain access to the DNA (27,52).

The hAR AF1 and AF2 functions can both be stimulated by p160 proteins. Our observation and those of others (26, 40, 53) that the LBD of the hAR has no intrinsic AF2 transcription activationfunction does not entirely fit into this model and prompted usto study the role of p160 proteins in the functioning of thisreceptor in more detail. Cotransfection experiments in COS cellsand in CV-1 cells with the isolated NTD and LBD revealed thatthe AF1 function can be stimulated by 160-kDa NR coactivatorsand that, only under the conditions of p160 overexpression, theLBD displays a transcription activation function that has allthe characteristics of a classical AF2. The fact that the LBDhas no measurable AF2 activity in the absence of ectopically expressedcoactivator is consistent with the observation that it has lowaffinity for SRC-1e in GST pull-down experiments. Under the sameconditions, the mER LBD binds well to SRC-1e, which explains thehigh intrinsic AF2 activity of this receptor (13). Such differencesin the affinities of distinct NR LBDs for coactivators have alsobee reported by others (14, 50, 72). Note that in most casesthe LBDs of receptors that have a strong intrinsic AF2 activity(such as ER, TR, RAR, and RXR) also display the highest affinityforcoactivators.

Using the yeast two-hybrid assay, Ding et al. (14) demonstrated that the hAR LBD fails to interact with the central NIRof SRC-1. Yet, in their experiments an interaction was seen withthe carboxy-terminal NR box IV that is specific to the SRC-1aisoform. We have not analyzed the interaction of the AR with SRC-1aor with a fragment containing the NR box IV in vitro, since ourfunctional data clearly demonstrate that SRC-1a is a less potentcoactivator for the hAR AF2 function than SRC-1e. In addition,Kalkhoven et al. (29) reported that the mutation of NR box IVdoes not affect the ability of SRC-1a to stimulate the transcriptionalactivity of the mER and Takeshita et al. (59) showed that, althoughthe TR can interact with NR box IV in GST pull-down experiments,this interaction is undetectable with DNA-bound TR. Together,these data raise the question of the physiological relevance ofthe LBD-box IV interaction. Recently, Hong et al. (22) identifiedan auxiliary region, specific to the GRIP1-TIF2 subgroup of coactivators,that is required for the efficient interaction of the GRIP1 NIRwith the AR LBD in yeast, thus providing yet another possibleexplanation of why we were unable to detect a strong LBD-SRC-1einteraction in GST pull down. However, our functional data demonstratethat both TIF2 and SRC-1e coactivate the hAR LBD, as well as thefull-size AR, to similar extents and thus suggest that both coactivatorsinteract with the receptor in similarways.

Contrary to the LBD, we saw a good physical interaction between the hAR NTD and SRC-1e. Likewise, weak but specific interactionsof SRC-1 with the NTD of the TR $beta$ (28) and of SRC-1 and TIF2with the NTD of the ER have been described (33, 66), and theprogesterone receptor (PR) LBD and NTD were both shown to interactin vitro with TIF2 and SRC-1 (46). Moreover, cotransfectionof SRC-1 stimulates the transcriptional activity of an ER moleculein which AF2 is mutated (54) and of the isolated AF1 functionsof the PR, GR, and ER (46, 66). We have not characterizedthe interaction of the hAR NTD with p160 proteins in more detail,but as for the ER NTD (66), the three LXXLL motifs that interactwith the LBD aredispensable.

A novel role for the NTD in the functioning of the native AR. Functional interactions between the hAR LBD and the NTD have been described in yeast and in mammalian cells (8, 15, 31).We demonstrate here that these domains physically interact inGST pull-down experiments. Since the NTD also interacts with coactivators,this suggests that a ternary complex of the NTD, the LBD, andcoactivators might exist, as could also be concluded from experimentsby others (24, 39, 46). From our GST pull-down data it remainsunclear whether the NTD and the LBD are engaged in a direct interactionor whether the pull down results from an indirect interactionmediated by a third partner present in the cell extract, whichwould act as a bridging factor. Although p160 proteins have beensuggested to build a "molecular bridge" between the NTD and theLBD (24, 39), two observations argue against such a model.Firstly, the NTD-LBD interaction can be demonstrated in the yeastdouble-hybrid system (8, 15), although yeast cells lack functionalhomologues of p160 coactivators. Secondly, the AF1a mutation hasno effect on the functional interaction between the NTD and p160proteins. Thus, if p160 coactivators acted as bridging factors,one would expect the NTD-LBD interaction to be unaffected by thismutation. Our GST pull-down and mammalian two-hybrid experiments,however, demonstrate the opposite. Still, the involvement of other(yet unidentified) bridging factors in our cell lysates cannotbe excluded apriori.

The model that we propose is that the interaction of the hAR NTD with the LBD generates a novel platform for the recruitmentof coactivators to the receptor, which compensates for the lowintrinsic affinity of the isolated hAR LBD for coactivators. Theinteraction of coactivators with the native hAR would thus occurthrough both strong contacts with the NTD and weak contacts withthe LBD, and the apparent coactivator properties of the NTD forthe LBD result from the recruitment of endogenous coactivatorsto the NTD-LBD complex. Alternatively, the ligand-dependent bindingof the NTD to the LBD could relieve some inhibitory function locatedin the LBD. Although we do not have clear indications of an inhibitoryregion in the AR LBD, such function has been assigned to the carboxyterminus of the PR LBD (70).

The nature of the DBD influences the coactivator properties of TIF2 for the hAR LBD. Our observation that a DBD-LBD construct is activated efficiently by both p160 proteins and the NTD whereas G4-LBD is activatedefficiently only by the NTD suggests that the mode of interactionof coactivators with the LBD, in the absence of NTD, differs fromthe binding of the NTD to the LBD. Possibly, DNA binding throughthe homologous DBD induces subtle conformational changes in theLBD that are essential for efficient binding of coactivators.Alternatively, dimers of functional AF2 domains are essentialfor the interaction of SCR-1e with the LBD (29), and the conformationof a DBD-LBD homodimer could differ from that of a G4-LBD homodimer.Although the hAR contains a leucine-rich motif comparable to theone that is essential for dimerization in the ER (16), its maindimerization interface resides within the second zinc finger ofthe DBD (68). Thus, in the GAL-LBD homodimer, dimerization canbe assumed to occur through the GAL4 DBD, resulting in a suboptimalalignment of the LBDs, whereas the DBD-LBD construct dimerizeson DNA through the hAR DBD, resulting in a dimer that efficientlybinds coactivators. Yet another possibility is that the hAR DBDalso binds accessory proteins, such as p/CAF (9) or small nuclearRING finger protein (41), which could cooperate with the p160proteins to stimulatetranscription.

Mutation in the hAR LBD and NTD and their effects on transcriptional activity. We generated point mutations in the hAR to validate the above-described model. A conserved lysine residue at the distal endof H3 of the LBD was shown to be essential for interaction withcoactivators and for high intrinsic AF2 activity in many NRs (17,20, 42, 43). When this mutation is introduced in a DBD-LBDconstruct, it dramatically reduces the coactivator propertiesof TIF2 for the hAR AF2, similar to the effects described forthe ER and the TR. However, the interaction with the NTD remainsintact. Thus, the K720A mutation discriminates between the interactionof the LBD with either p160 proteins or the NTD. Since this mutationhas no severe effects on the transcriptional activity of the full-sizehAR, this result indicates that in the native receptor the reducedinteraction of the coactivators with the LBD can be compensatedfor by additional interactions, for instance, with the NTD. Theobservation that the full-size ER carrying the corresponding mutationis transcriptionally inactive (20) and that the activity ofthe TR is reduced to ~40% (17) indicates that for these receptorsthe contacts between the LBD and the coactivators are crucial,whereas for the hAR their contribution is of minor importance,relative to the NTD-coactivatorinteractions.

Contrary to the K720A exchange, the mutation of two bulky hydrophobic residues in H12 (I898A/I899A) (13) completely destroysall transcriptional activity of the full-size hAR and impairsthe interaction of the isolated LBD with both p160 proteins andthe hAR NTD. Similar effects are observed when an adjacent conservedglutamate is mutated to a glutamine (8) or when the LBD isoccupied by the antagonist hydroxyflutamide (our unpublished results).Yet, the mutated receptor is activated by overexpression of p160proteins, similar to the effects observed with an ER moleculein which AF2 is mutated (33). These effects could be due tothe binding of the coactivator to the intactNTD.

The mutation of isoleucine 182 and leucine 183 to alanines dramatically impairs the activity of the full-size receptor (11).This effect can be explained by the observation that the functionaland physical interactions between the NTD and the LBD are impaired,thus not allowing the efficient recruitment of coactivators tothe mutated full-size receptor. In addition, the NTD and p160coactivators cooperatively stimulate the transcriptional activityof the hAR LBD, when expressed simultaneously, as was also demonstratedfor the PR (46). The importance of the AF1a region is furtherunderlined by the observation that this cooperativity fully relieson an intact AF1a domain. Two other mutations in the AR LBD weredescribed that cause androgen insensitivity and that affect theNTD-LBD interaction (32) (V889M and R752Q). At physiologicalhormone concentrations, the transcriptional activity of a receptormolecule carrying one of these mutations is considerably lowerthan that of the native receptor, and efficient transactivationoccurs only at 10³- to 10⁴-fold-higher androgen concentrations. According to our model,the disruption of the NTD-LBD interaction by these mutations wouldnot allow the efficient binding of coactivators, resulting ina deficient receptor and androgeninsensitivity.

Deletion-mapping experiments were performed previously (8, 31) to define the region of the hAR NTD that binds to theLBD. These results indicated that the extreme NH₂ terminus (aminoacids 15 to 30) is essential for this interaction. Earlier reportedresults, however, showed that a receptor devoid of the first 142residues still retains 70% of the activity of the native protein(26). Our observation that the mutation of AF1a also affectsthe binding of the hAR NTD to the LBD demonstrates that the extremeNH₂ terminus alone is not sufficient for this interaction andsuggests that an extended region of the NTD is required, as wasalso suggested by Ikonen et al. (24). Moreover, in additionto a correctly folded LBD, the interaction most likely also requiresthe correct folding of the NTD. The introduction of point mutations,as we did in this study, probably has less severe effects on thethree-dimensional structure of the different domains of the receptorthan the deletion of large parts of the protein described in otherstudies (8, 31) and would therefore better conserve the originalconformation of theprotein.

Mutation of the three LXXLL motifs in p160 proteins and the effect on their coactivator activity for the hAR. We also analyzed the effects of mutations in the three conserved LXXLL motifs in p160 coactivators and found that these mutatedproteins can still stimulate the transcriptional activity of thenative hAR, although to a slightly lesser extent than the wild-typecoactivators. Nevertheless, their coactivator properties for theisolated LBD are dramatically impaired, so the residual effectthat is seen with the full-size receptor results from their coactivatoractivity on the NTD and strengthens the hypothesis that the interactionof p160 proteins with the NTD-LBD complex in the full-size receptorcan occur through residues outside of the NIR. In addition, thecooperativity between the NTD and TIF2 for the stimulation ofthe transcriptional activity of the hAR LBD is conserved witha TIF2 molecule in which the three NR boxes are mutated. The observationthat similar mutations have more severe effects on the coactivatorproperties for the ER, PPAR, RXR, and GR (29, 46) is yet anotherindication that for these receptors the contribution of the LBDto the interaction with coactivators is most important. For thehAR, however, the AF2 function is much less prominent, while theAF1 function (and thus the NTD) is the major contributor to thetotal transcriptionalactivity.

	ACKNOWLEDGMENTS

We thank A. O. Brinkmann, H. Gronemeyer, M. G. Parker, S. Plaisance, and H. Stunnenberg for the generous gifts of plasmids;R. Bollen and H. De Bruyn for excellent technical assistance;and V. Feytons for the expert synthesis ofoligonucleotides.

This work was supported by a grant from Geconcerteerde Onderzoeksactie van de Vlaamse Gemeenschap, by grants from the BelgianFonds voor Geneeskundig Wetenschappelijk Onderzoek, and by a grantfrom the Interuniversity Poles of Attraction Programme, BelgianState, Prime Minister's Office, Federal Office for Scientific,Technical and Cultural Affairs. F.C. is a Senior Research Assistantof the Fund for Scientific Research Flanders(Belgium).

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Biochemistry, Campus Gasthuisberg, Herestraat 49, B-3000 Leuven, Belgium.Phone: 32 16 34 57 08. Fax: 32 16 34 59 95. E-mail: Ben.Peeters{at}med.kuleuven.ac.be.

Present address: Laboratory for Molecular Oncology, Centre for Human Genetics, University of Leuven, B-3000 Leuven,Belgium.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Aarnisalo, P., J. J. Palvimo, and O. A. Jänne. 1998. CREB-binding protein in androgen receptor-mediated signaling. Proc. Natl. Acad. Sci. USA 95:2122-2127[Abstract/Free Full Text].

2. Alen, P., F. Claessens, E. Schoenmakers, J. V. Swinnen, G. Verhoeven, W. Rombauts, and B. Peeters. 1999. Interaction of the putative androgen receptor-specific coactivator ARA₇₀/ELE1 $alpha$ with multiple steroid receptors and identification of an internally deleted ELE1 $beta$ isoform. Mol. Endocrinol. 13:117-128[Abstract/Free Full Text].

3. Anzick, S. L., J. Kononen, R. L. Walker, D. O. Azorsa, M. M. Tanner, X. Y. Guan, G. Sauter, O. P. Kallioniemi, J. M. Trent, and P. S. Meltzer. 1997. AIB1, a steroid receptor coactivator amplified in breast and ovarian cancer. Science 277:965-968[Abstract/Free Full Text].

4. Baniahmad, A., A. C. Kohne, and R. Renkawitz. 1992. A transferable silencing domain is present in the thyroid hormone receptor, in the v-erbA oncogene product and in the retinoic acid receptor. EMBO J. 11:1015-1023[Medline].

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

6. Beato, M., S. Chavez, and M. Truss. 1996. Transcriptional regulation by steroid hormones. Steroids 61:240-251[Medline].

7. Beato, M., and A. Sanchez-Pacheco. 1996. Interaction of steroid hormone receptors with the transcription initiation complex. Endocrine Rev. 17:587-609[Abstract/Free Full Text].

8. Berrevoets, C. A., P. Doesburg, K. Steketee, J. Trapman, and A. O. Brinkmann. 1998. Functional interactions of the AF-2 activation domain core region of the human androgen receptor with the amino-terminal domain and with the transcriptional coactivator TIF2 (transcriptional intermediary factor 2). Mol. Endocrinol. 12:1172-1183[Abstract/Free Full Text].

9. Blanco, J. C. G., S. Minucci, J. Lu, X. J. Yang, K. K. Walker, H. Chen, R. M. Evans, Y. Nakatani, and K. Ozato. 1998. The histone acetylase PCAF is a nuclear receptor coactivator. Genes Dev. 12:1638-1651[Abstract/Free Full Text].

10. Buchert, M., S. Schneider, M. T. Adams, H. P. Hefti, K. Moelling, and C. M. Hovens. 1997. Useful vectors for the two-hybrid system in mammalian cells. BioTechniques 23:396-402[Medline].

11. Chamberlain, N. L., D. C. Whitacre, and R. L. Miesfeld. 1996. Delineation of two distinct type 1 activation functions in the androgen receptor amino-terminal domain. J. Biol. Chem. 271:26772-26778[Abstract/Free Full Text].

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

13. Danielian, P. S., R. White, J. A. Lees, and M. G. Parker. 1992. Identification of a conserved region required for hormone dependent transcriptional activation by steroid hormone receptors. EMBO J. 11:1025-1033[Medline].

14. Ding, X. F., C. M. Anderson, H. Ma, H. Hong, R. M. Uht, P. Kushner, and M. R. Stallcup. 1998. Nuclear receptor-binding sites of coactivators glucocorticoid receptor interaction protein 1(GRIP1) and steroid receptor coactivator 1 (SRC1): multiple motifs with different binding specificities. Mol. Endocrinol. 12:302-313[Abstract/Free Full Text].

15. Doesburg, P., C. W. Kuil, C. A. Berrevoets, K. Steketee, P. W. Faber, E. Mulder, A. O. Brinkmann, and J. Trapman. 1997. Functional in vivo interaction between the amino-terminal and the ligand binding domain of the androgen receptor. Biochemistry 36:1052-1064[Medline].

16. Fawell, S. E., J. A. Lees, R. White, and M. G. Parker. 1990. Characterization and colocalization of steroid binding and dimerization activities in the mouse estrogen receptor. Cell 60:953-962[Medline].

17. Feng, W., R. C. J. Ribeiro, R. L. Wagner, H. Nguyen, J. W. Apriletti, R. J. Fletterick, J. D. Baxter, P. J. Kushner, and B. L. West. 1998. Hormone-dependent coactivator binding to a hydrophobic cleft on nuclear receptors. Science 280:1747-1749[Abstract/Free Full Text].

18. Fronsdal, K., N. Engedal, T. Slagsvold, and F. Saatcioglu. 1998. CREB binding protein is a coactivator for the androgen receptor and mediates cross-talk with AP-1. J. Biol. Chem. 273:31853-31859[Abstract/Free Full Text].

19. Heery, D. M., E. Kalkhoven, S. Hoare, and M. G. Parker. 1997. A signature motif in transcriptional co-activators mediates binding to nuclear receptors. Nature 387:733-736[Medline].

20. Henttu, P. M. A., E. Kalkhoven, and M. G. Parker. 1997. AF-2 activity and recruitment of steroid receptor coactivator 1 to the estrogen receptor depend on a lysine residue conserved in nuclear receptors. Mol. Cell. Biol. 17:1832-1839[Abstract].

21. Hong, H., K. Kohli, M. J. Garabedian, and M. R. Stallcup. 1997. GRIP1, a transcriptional coactivator for the AF-2 transactivation domain of steroid, thyroid, retinoid, and vitamin D receptors. Mol. Cell. Biol. 17:2735-2744[Abstract].

22. Hong, H., B. D. Darimont, H. Ma, L. Yang, K. R. Yamamoto, and M. R. Stallcup. 1999. An additional region of coactivator GRIP1 required for interaction with the hormone-binding domains of a subset of nuclear receptors. J. Biol. Chem. 274:3496-3502[Abstract/Free Full Text].

23. Horwitz, K. B., T. A. Jackson, D. L. Bain, J. K. Richer, G. S. Takimoto, and L. Tung. 1996. Nuclear receptor coactivators and corepressors. Mol. Endocrinol. 10:1167-1177[Abstract/Free Full Text].

24. Ikonen, T., J. J. Palvimo, and O. A. Jänne. 1997. Interaction between the amino- and carboxyl-terminal regions of the rat androgen receptor modulates transcriptional activity and is influenced by nuclear receptor coactivators. J. Biol. Chem. 272:29821-29828[Abstract/Free Full Text].

25. Jenster, G., H. A. G. M. van der Korput, C. C. J. van Groonhoven, T. H. Van der Kwast, J. Trapman, and A. O. Brinkmann. 1991. Domains of the human androgen receptor involved in steroid binding, transcriptional activation, and subcellular localization. Mol. Endocrinol. 5:1396-1404[Abstract/Free Full Text].

26. Jenster, G., H. A. G. M. van der Korput, J. Trapman, and A. O. Brinkmann. 1995. Identification of two transcription activation units in the N-terminal domain of the human androgen receptor. J. Biol. Chem. 270:7341-7346[Abstract/Free Full Text].

27. Jenster, G. 1998. Coactivators and corepressors as mediators of nuclear receptor function: an update. Mol. Cell. Endocrinol. 143:1-7[Medline].

28. Jeyakumar, M., M. R. Tanen, and M. K. Bagchi. 1997. Analysis of the functional role of steroid receptor coactivator-1 in ligand-induced transactivation by thyroid hormone receptor. Mol. Endocrinol. 11:755-767[Abstract/Free Full Text].

29. Kalkhoven, E., J. E. Valentin, D. M. Heery, and M. G. Parker. 1998. Isoforms of steroid receptor co-activator 1 differ in their ability to potentiate transcription by the oestrogen receptor. EMBO J. 17:232-243[Medline].

30. Kamei, Y., L. Xu, T. Heinzel, J. Torchia, R. Kurokawa, B. Gloss, S.-C. Lin, R. A. Heyman, D. W. Rose, C. K. Glass, and M. G. Rosenfeld. 1996. A CBP integrator complex mediates transcriptional activation and AP-1 inhibition by nuclear receptors. Cell 85:403-414[Medline].

31. Langley, E., Z. X. Zhou, and E. M. Wilson. 1995. Evidence for an anti-parallel orientation of the ligand-activated human androgen receptor dimer. J. Biol. Chem. 270:29983-29990[Abstract/Free Full Text].

32. Langley, E., J. A. Kemppainen, and E. M. Wilson. 1998. Intermolecular NH₂-carboxyl-terminal interactions in androgen receptor dimerization revealed by mutations that cause androgen insensitivity. J. Biol. Chem. 273:92-101[Abstract/Free Full Text].

33. Lavinsky, R. M., K. Jepsen, T. Heinzel, J. Torchia, T.-M. Mullen, R. Schiff, A. L. Del-Rio, M. Ricolte, S. Ngo, J. Gemsch, S. G. Hilsenbeck, C. K. Osborne, C. K. Glass, M. G. Rosenfeld, and D. W. Rose. 1998. Diverse signaling pathways modulate nuclear receptor recruitment of N-CoR and SMRT complexes. Proc. Natl. Acad. Sci. USA 95:2920-2925[Abstract/Free Full Text].

34. Leers, J., E. Treuter, and J. A. Gustaffson. 1998. Mechanistic principles in NR box-dependent interaction between nuclear hormone receptors and the coactivator TIF2. Mol. Cell. Biol. 18:6001-6013[Abstract/Free Full Text].

35. Li, H., P. J. Gomes, and D. J. Chen. 1996. RAC3, a steroid/nuclear receptor-associated coactivator that is related to SRC-1 and TIF2. Proc. Natl. Acad. Sci. USA 94:8479-8484[Abstract/Free Full Text].

36. Li, H., and D. Chen. 1998. The receptor-associated coactivator 3 activates transcription through CREB-binding protein recruitment and autoregulation. J. Biol. Chem. 273:5948-5954[Abstract/Free Full Text].

37. Mangelsdorf, D. J., C. Thummel, M. Beato, P. Herrlich, G. Schutz, K. Umesono, B. Blumberg, P. Kastner, M. Mark, P. Chambon, and R. Evans. 1995. The nuclear receptor superfamily: the second decade. Cell 83:835-839[Medline].

38. Marivoet, S., M. Hertogen, G. Verhoeven, and W. Heyns. 1990. Antibodies against synthetic peptide recognise the human and rat androgen receptor. J. Steroid Biochem. Mol. Biol. 37:39-45[Medline].

39. McInerney, E. M., M. J. Tsai, B. W. O'Malley, and B. S. Katzenellenbogen. 1996. Analysis of estrogen receptor transcriptional enhancement by a nuclear hormone receptor coactivator. Proc. Natl. Acad. Sci. USA 93:10069-10073[Abstract/Free Full Text].

40. Moilanen, A., N. Rouleau, T. Ikonen, J. J. Palvimo, and O. A. Jänne. 1997. The presence of a transcription activation function in the hormone-binding domain of androgen receptor is revealed by studies in yeast cells. FEBS Lett. 412:355-358[Medline].

41. Moilanen, A., H. Poukka, U. Karvonen, M. Häkli, O. A. Jänne, and J. J. Palvimo. 1998. Identification of a novel RING finger protein as a coregulator in steroid receptor-mediated gene transcription. Mol. Cell. Biol. 18:5128-5139[Abstract/Free Full Text].

42. Moras, D., and H. Gronemeyer. 1998. The nuclear receptor ligand-binding domain: structure and function. Curr. Opin. Cell Biol. 10:384-391[Medline].

43. Nolte, R. T., G. B. Wisely, S. Westin, J. E. Cobb, M. Lambert, R. Kurokawa, M. Rosenfeld, T. M. Willson, C. K. Glass, and M. V. Milburn. 1998. Ligand binding and co-activator assembly of the peroxisome proliferator-activated receptor- $gamma$ . Nature 395:137-143[Medline].

44. 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[Medline].

45. Onate, S. A., S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1995. Sequence and characterization of a coactivator for the steroid hormone receptor superfamily. Science 270:1354-1357[Abstract/Free Full Text].

46. Onate, S. A., V. Boonyaratanakornkit, T. E. Spencer, S. Y. Tsai, M. J. Tsai, D. P. Edwards, and B. W. O'Malley. 1998. The steroid receptor coactivator-1 contains multiple receptor interaction domains that cooperatively enhance the activation function 1 (AF1) and AF2 domains of steroid receptors. J. Biol. Chem. 273:12101-12108[Abstract/Free Full Text].

47. Parker, M. G., and R. White. 1996. Nuclear receptors spring into action. Nat. Struct. Biol. 3:113-115[Medline].

48. Plaisance, S., W. VandenBerghe, E. Boone, W. Fiers, and G. Haegeman. 1997. Recombination signal sequence binding protein J kappa is constitutively bound to the NF-kappa B site of the interleukin-6 promoter and acts as a negative regulatory factor. Mol. Cell. Biol. 17:3733-3743[Abstract].

49. Quigley, C. A., A. De Bellis, K. B. Marschke, M. K. El-Awady, E. M. Wilson, and F. S. French. 1995. Androgen receptor defects: historical, clinical, and molecular perspectives. Endocrine Rev. 16:271-321[Abstract/Free Full Text].

50. Schmidt, S., A. Baniahmad, M. Eggert, S. Schneider, and R. Renkawitz. 1998. Multiple receptor interaction domains of GRIP1 function in synergy. Nucleic Acids. Res. 26:1191-1197[Abstract/Free Full Text].

51. Shiau, A. K., D. Barstad, P. M. Loria, L. Cheng, P. J. Kushner, D. A. Agard, and G. L. Greene. 1999. The structural basis of estrogen receptor/coactivator recognition and the antagonism of this interaction by tamoxifen. Cell 95:927-937.

52. Shibata, H., T. E. Spencer, S. A. Onate, G. Jenster, S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1997. Role of coactivators and corepressors in the mechanism of steroid/thyroid receptor action. Recent Prog. Horm. Res. 52:141-165.

53. Simental, J. A., M. Sar, and E. M. Wilson. 1992. Domain functions of the androgen receptor. J. Steroid Biochem. Mol. Biol. 43:37-41[Medline].

54. Smith, C. L., Z. Nawaz, and B. W. O'Malley. 1997. Coactivator and corepressor regulation of the agonist/antagonist activity of the mixed antiestrogen, 4-hydroxytamoxifen. Mol. Endocrinol. 11:657-666[Abstract/Free Full Text].

55. 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[Medline].

56. Suen, C. S., T. J. Berrodin, R. Mastroeni, B. J. Cheskis, C. R. Lyttle, and D. E. Frail. 1998. A transcriptional coactivator, steroid receptor coactivator-3, selectively augments steroid receptor transcriptional activity. J. Biol. Chem. 273:27645-27653[Abstract/Free Full Text].

57. Takeshita, A., P. M. Yen, S. Misti, G. R. Cardona, Y. Liu, and W. W. Chin. 1996. Molecular cloning and properties of a full-length putative thyroid hormone receptor coactivator. Endocrinology 137:3594-3597[Abstract].

58. Takeshita, A., G. R. Cardona, N. Koibuchi, C. S. Suen, and W. W. Chin. 1997. TRAM-1, a novel 160-kDa thyroid hormone receptor activator molecule, exhibits distinct properties from steroid receptor coactivator-1. J. Biol. Chem. 272:27629-27634[Abstract/Free Full Text].

59. Takeshita, A., P. M. Yen, M. Ikeda, G. R. Cardona, Y. Liu, N. Koibuchi, E. R. Norwitz, and W. W. Chin. 1998. Thyroid hormone response elements differentially modulate the interactions of thyroid hormone receptors with two receptor binding domains in the steroid receptor coactivator-1. J. Biol. Chem. 273:21554-21562[Abstract/Free Full Text].

60. Torchia, J., D. W. Rose, J. Inostroza, Y. Kamei, S. Westin, C. Glass, and M. G. Rosenfeld. 1997. The transcriptional co-activator p/CIP binds CBP and mediates nuclear-receptor function. Nature 387:677-684[Medline].

61. Torchia, J., C. Glass, and M. Rosenfeld. 1998. Co-activators and co-repressors in the integration of transcriptional responses. Curr. Opin. Cell. Biol. 10:373-383[Medline].

62. Tsai, M. J., and B. W. O'Malley. 1994. Molecular mechanisms of action of steroid/thyroid receptor superfamily members. Annu. Rev. Biochem. 63:451-486[Medline].

63. Tsai, R. Y. L., and R. R. Reed. 1997. Using a eukaryotic GST fusion vector for proteins difficult to express in E. coli. BioTechniques 23:794-800[Medline].

64. Voegel, J. J., M. J. S. Heine, C. Zechel, P. Chambon, and H. Gronemeyer. 1996. TIF2, a 160 kDa transcriptional mediator for the ligand-dependent activation function AF-2 of nuclear receptors. EMBO J. 15:3667-3675[Medline].

65. Voegel, J. J., M. J. S. Heine, M. Tini, V. Vivat, P. Chambon, and H. Gronemeyer. 1998. The coactivator TIF2 contains three nuclear receptor-binding motifs and mediates transactivation through CBP binding-dependent and -independent pathways. EMBO J. 17:507-519[Medline].

66. Webb, P., P. Nguyen, J. Shinsako, C. Anderson, W. Feng, M. P. Nguyen, D. Chen, S. M. Huang, S. Subramanian, E. McKinerney, B. S. Katzenellenbogen, M. R. Stallcup, and P. J. Kushner. 1998. Estrogen receptor activation function 1 works by binding p160 coactivator proteins. Mol. Endocrinol. 12:1605-1618[Abstract/Free Full Text].

67. Williams, S. P., and P. B. Sigler. 1998. Atomic structure of progesterone complexed with its receptor. Nature 393:392-396[Medline].

68. Wong, C. I., Z. X. Zhou, M. Sar, and E. M. Wilson. 1993. Steroid requirements for androgen receptor dimerization and DNA binding. J. Biol. Chem. 268:19004-19012[Abstract/Free Full Text].

69. Wurtz, J. M., W. Bourguet, J. P. Renaud, V. Vivat, P. Chambon, D. Moras, and H. Gronemeyer. 1996. A canonical structure for the ligand-binding domain of nuclear receptors. Nat. Struct. Biol. 3:87-94[Medline].

70. Xu, J., Z. Nawaz, S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1996. The extreme C-terminus of the progesterone receptor contains a transcriptional repressor domain that functions through a putative corepressor. Proc. Natl. Acad. Sci. USA 93:12195-12199[Abstract/Free Full Text].

71. Yang, X. J., V. V. Ogryzko, J. I. Nishikawa, B. Howard, and Y. Nakatani. 1996. A p300/CBP-associated factor that competes with the adenoviral oncoprotein E1A. Nature 283:319-324.

72. Zhou, G., R. Cummings, Y. Li, S. Mitra, H. A. Wilkinson, A. Elbrecht, J. D. Hermes, J. M. Schaeffer, R. G. Smith, and D. E. Moller. 1998. Nuclear receptors have distinct affinities for coactivators: characterization by fluorescence resonance energy transfer. Mol. Endocrinol. 12:1594-1604[Abstract/Free Full Text].

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Haelens, A., Tanner, T., Denayer, S., Callewaert, L., Claessens, F. (2007). The Hinge Region Regulates DNA Binding, Nuclear Translocation, and Transactivation of the Androgen Receptor. Cancer Res. 67: 4514-4523 [Abstract] [Full Text]
Moehren, U., Papaioannou, M., Reeb, C. A., Hong, W., Baniahmad, A. (2007). Alien Interacts with the Human Androgen Receptor and Inhibits Prostate Cancer Cell Growth. Mol. Endocrinol. 21: 1039-1048 [Abstract] [Full Text]
Yang, Z., Chang, Y.-J., Miyamoto, H., Yeh, S., Yao, J. L., di Sant'Agnese, P. A., Tsai, M.-Y., Chang, C. (2007). Suppression of Androgen Receptor Transactivation and Prostate Cancer Cell Growth by Heterogeneous Nuclear Ribonucleoprotein A1 via Interaction with Androgen Receptor Coregulator ARA54. Endocrinology 148: 1340-1349 [Abstract] [Full Text]
Yang, Z., Chang, Y.-J., Miyamoto, H., Ni, J., Niu, Y., Chen, Z., Chen, Y.-L., Yao, J. L., di Sant'Agnese, P. A., Chang, C. (2007). Transgelin Functions as a Suppressor via Inhibition of ARA54-Enhanced Androgen Receptor Transactivation and Prostate Cancer Cell Growth. Mol. Endocrinol. 21: 343-358 [Abstract] [Full Text]
Burd, C. J, Morey, L. M, Knudsen, K. E (2006). Androgen receptor corepressors and prostate cancer. Endocr Relat Cancer 13: 979-994 [Abstract] [Full Text]
Dehm, S. M., Tindall, D. J. (2006). Ligand-independent Androgen Receptor Activity Is Activation Function-2-independent and Resistant to Antiandrogens in Androgen Refractory Prostate Cancer Cells. J. Biol. Chem. 281: 27882-27893 [Abstract] [Full Text]
Wu, Y., Kawate, H., Ohnaka, K., Nawata, H., Takayanagi, R. (2006). Nuclear Compartmentalization of N-CoR and Its Interactions with Steroid Receptors.. Mol. Cell. Biol. 26: 6633-6655 [Abstract] [Full Text]
Ma, A.-H., Xia, L., Desai, S. J., Boucher, D. L., Guan, Y., Shih, H.-M., Shi, X.-B., deVere White, R. W., Chen, H.-W., Tepper, C. G., Kung, H.-J. (2006). Male Germ Cell-Associated Kinase, a Male-Specific Kinase Regulated by Androgen, Is a Coactivator of Androgen Receptor in Prostate Cancer Cells.. Cancer Res. 66: 8439-8447 [Abstract] [Full Text]
Tian, H., Mahajan, M. A., Wong, C. T., Habeos, I., Samuels, H. H. (2006). The N-Terminal A/B Domain of the Thyroid Hormone Receptor-{beta}2 Isoform Influences Ligand-Dependent Recruitment of Coactivators to the Ligand-Binding Domain. Mol. Endocrinol. 20: 2036-2051 [Abstract] [Full Text]
Yoon, H.-G., Wong, J. (2006). The Corepressors Silencing Mediator of Retinoid and Thyroid Hormone Receptor and Nuclear Receptor Corepressor Are Involved in Agonist- and Antagonist-Regulated Transcription by Androgen Receptor. Mol. Endocrinol. 20: 1048-1060 [Abstract] [Full Text]
Li, J., Fu, J., Toumazou, C., Yoon, H.-G., Wong, J. (2006). A Role of the Amino-Terminal (N) and Carboxyl-Terminal (C) Interaction in Binding of Androgen Receptor to Chromatin. Mol. Endocrinol. 20: 776-785 [Abstract] [Full Text]
Georget, V., Bourguet, W., Lumbroso, S., Makni, S., Sultan, C., Nicolas, J.-C. (2006). Glutamic Acid 709 Substitutions Highlight the Importance of the Interaction between Androgen Receptor Helices H3 and H12 for Androgen and Antiandrogen Actions. Mol. Endocrinol. 20: 724-734 [Abstract] [Full Text]
Zheng, Z., Cai, C., Omwancha, J., Chen, S.-Y., Baslan, T., Shemshedini, L. (2006). SUMO-3 Enhances Androgen Receptor Transcriptional Activity through a Sumoylation-independent Mechanism in Prostate Cancer Cells. J. Biol. Chem. 281: 4002-4012 [Abstract] [Full Text]
Callewaert, L., Van Tilborgh, N., Claessens, F. (2006). Interplay between Two Hormone-Independent Activation Domains in the Androgen Receptor. Cancer Res. 66: 543-553 [Abstract] [Full Text]
Xiao, F., Mirwald, A., Papaioannou, M., Baniahmad, A., Klug, J. (2005). Secretoglobin 2A1 Is under Selective Androgen Control Mediated by a Peculiar Binding Site for Sp Family Transcription Factors. Mol. Endocrinol. 19: 2964-2978 [Abstract] [Full Text]
Agoulnik, I. U., Vaid, A., Bingman, W. E. III, Erdeme, H., Frolov, A., Smith, C. L., Ayala, G., Ittmann, M. M., Weigel, N. L. (2005). Role of SRC-1 in the Promotion of Prostate Cancer Cell Growth and Tumor Progression. Cancer Res. 65: 7959-7967 [Abstract] [Full Text]
Zhang, Y., Wang, X.-W., Jelovac, D., Nakanishi, T., Yu, M.-h., Akinmade, D., Goloubeva, O., Ross, D. D., Brodie, A., Hamburger, A. W. (2005). The ErbB3-binding protein Ebp1 suppresses androgen receptor-mediated gene transcription and tumorigenesis of prostate cancer cells. Proc. Natl. Acad. Sci. USA 102: 9890-9895 [Abstract] [Full Text]
Ye, X., Han, S. J., Tsai, S. Y., DeMayo, F. J., Xu, J., Tsai, M.-J., O'Malley, B. W. (2005). Roles of steroid receptor coactivator (SRC)-1 and transcriptional intermediary factor (TIF) 2 in androgen receptor activity in mice. Proc. Natl. Acad. Sci. USA 102: 9487-9492 [Abstract] [Full Text]
Burd, C. J., Petre, C. E., Moghadam, H., Wilson, E. M., Knudsen, K. E. (2005). Cyclin D1 Binding to the Androgen Receptor (AR) NH2-Terminal Domain Inhibits Activation Function 2 Association and Reveals Dual Roles for AR Corepression. Mol. Endocrinol. 19: 607-620 [Abstract] [Full Text]
Hodgson, M. C., Astapova, I., Cheng, S., Lee, L. J., Verhoeven, M. C., Choi, E., Balk, S. P., Hollenberg, A. N. (2005). The Androgen Receptor Recruits Nuclear Receptor CoRepressor (N-CoR) in the Presence of Mifepristone via Its N and C Termini Revealing a Novel Molecular Mechanism for Androgen Receptor Antagonists. J. Biol. Chem. 280: 6511-6519 [Abstract] [Full Text]
Cho, S., Kagan, B. L., Blackford, J. A. Jr., Szapary, D., Simons, S. S. Jr. (2005). Glucocorticoid Receptor Ligand Binding Domain Is Sufficient for the Modulation of Glucocorticoid Induction Properties by Homologous Receptors, Coactivator Transcription Intermediary Factor 2, and Ubc9. Mol. Endocrinol. 19: 290-311 [Abstract] [Full Text]
Masiello, D., Chen, S.-Y., Xu, Y., Verhoeven, M. C., Choi, E., Hollenberg, A. N., Balk, S. P. (2004). Recruitment of {beta}-Catenin by Wild-Type or Mutant Androgen Receptors Correlates with Ligand-Stimulated Growth of Prostate Cancer Cells. Mol. Endocrinol. 18: 2388-2401 [Abstract] [Full Text]
Dubbink, H. J., Hersmus, R., Verma, C. S., van der Korput, H. A. G. M., Berrevoets, C. A., van Tol, J., Ziel-van der Made, A. C. J., Brinkmann, A. O., Pike, A. C. W., Trapman, J. (2004). Distinct Recognition Modes of FXXLF and LXXLL Motifs by the Androgen Receptor. Mol. Endocrinol. 18: 2132-2150 [Abstract] [Full Text]
Fu, M., Rao, M., Wu, K., Wang, C., Zhang, X., Hessien, M., Yeung, Y.-G., Gioeli, D., Weber, M. J., Pestell, R. G. (2004). The Androgen Receptor Acetylation Site Regulates cAMP and AKT but Not ERK-induced Activity. J. Biol. Chem. 279: 29436-29449 [Abstract] [Full Text]
Jang, H. D., Yoon, K., Shin, Y. J., Kim, J., Lee, S. Y. (2004). PIAS3 Suppresses NF-{kappa}B-mediated Transcription by Interacting with the p65/RelA Subunit. J. Biol. Chem. 279: 24873-24880 [Abstract] [Full Text]
Callewaert, L., Verrijdt, G., Haelens, A., Claessens, F. (2004). Differential Effect of Small Ubiquitin-Like Modifier (SUMO)-ylation of the Androgen Receptor in the Control of Cooperativity on Selective Versus Canonical Response Elements. Mol. Endocrinol. 18: 1438-1449 [Abstract] [Full Text]
Wang, Q., Udayakumar, T. S., Vasaitis, T. S., Brodie, A. M., Fondell, J. D. (2004). Mechanistic Relationship between Androgen Receptor Polyglutamine Tract Truncation and Androgen-dependent Transcriptional Hyperactivity in Prostate Cancer Cells. J. Biol. Chem. 279: 17319-17328 [Abstract] [Full Text]
Black, B. E., Vitto, M. J., Gioeli, D., Spencer, A., Afshar, N., Conaway, M. R., Weber, M. J., Paschal, B. M. (2004). Transient, Ligand-Dependent Arrest of the Androgen Receptor in Subnuclear Foci Alters Phosphorylation and Coactivator Interactions. Mol. Endocrinol. 18: 834-850 [Abstract] [Full Text]
Hosohata, K., Li, P., Hosohata, Y., Qin, J., Roeder, R. G., Wang, Z. (2003). Purification and Identification of a Novel Complex Which Is Involved in Androgen Receptor-Dependent Transcription. Mol. Cell. Biol. 23: 7019-7029 [Abstract] [Full Text]
Kasai, M., Guerrero-Santoro, J., Friedman, R., Leman, E. S., Getzenberg, R. H., DeFranco, D. B. (2003). The Group 3 LIM Domain Protein Paxillin Potentiates Androgen Receptor Transactivation in Prostate Cancer Cell Lines. Cancer Res. 63: 4927-4935 [Abstract] [Full Text]
Ghali, S. A., Gottlieb, B., Lumbroso, R., Beitel, L. K., Elhaji, Y., Wu, J., Pinsky, L., Trifiro, M. A. (2003). The Use of Androgen Receptor Amino/Carboxyl-Terminal Interaction Assays to Investigate Androgen Receptor Gene Mutations in Subjects with Varying Degrees of Androgen Insensitivity. J. Clin. Endocrinol. Metab. 88: 2185-2193 [Abstract] [Full Text]
Janssens, V., Jordens, J., Stevens, I., Van Hoof, C., Martens, E., De Smedt, H., Engelborghs, Y., Waelkens, E., Goris, J. (2003). Identification and Functional Analysis of Two Ca2+-binding EF-hand Motifs in the B"/PR72 Subunit of Protein Phosphatase 2A. J. Biol. Chem. 278: 10697-10706 [Abstract] [Full Text]
Callewaert, L., Verrijdt, G., Christiaens, V., Haelens, A., Claessens, F. (2003). Dual Function of an Amino-terminal Amphipatic Helix in Androgen Receptor-mediated Transactivation through Specific and Nonspecific Response Elements. J. Biol. Chem. 278: 8212-8218 [Abstract] [Full Text]
Liao, G., Chen, L.-Y., Zhang, A., Godavarthy, A., Xia, F., Ghosh, J. C., Li, H., Chen, J. D. (2003). Regulation of Androgen Receptor Activity by the Nuclear Receptor Corepressor SMRT. J. Biol. Chem. 278: 5052-5061 [Abstract] [Full Text]
Maira, M., Martens, C., Batsche, E., Gauthier, Y., Drouin, J. (2003). Dimer-Specific Potentiation of NGFI-B (Nur77) Transcriptional Activity by the Protein Kinase A Pathway and AF-1-Dependent Coactivator Recruitment. Mol. Cell. Biol. 23: 763-776 [Abstract] [Full Text]
Kumar, R., Thompson, E. B. (2003). Transactivation Functions of the N-Terminal Domains of Nuclear Hormone Receptors: Protein Folding and Coactivator Interactions. Mol. Endocrinol. 17: 1-10 [Abstract] [Full Text]
Christiaens, V., Bevan, C. L., Callewaert, L., Haelens, A., Verrijdt, G., Rombauts, W., Claessens, F. (2002). Characterization of the Two Coactivator-interacting Surfaces of the Androgen Receptor and Their Relative Role in Transcriptional Control*. J. Biol. Chem. 277: 49230-49237 [Abstract] [Full Text]
Wang, Q., Sharma, D., Ren, Y., Fondell, J. D. (2002). A Coregulatory Role for the TRAP-Mediator Complex in Androgen Receptor-mediated Gene Expression. J. Biol. Chem. 277: 42852-42858 [Abstract] [Full Text]
Reid, J., Murray, I., Watt, K., Betney, R., McEwan, I. J. (2002). The Androgen Receptor Interacts with Multiple Regions of the Large Subunit of General Transcription Factor TFIIF. J. Biol. Chem. 277: 41247-41253 [Abstract] [Full Text]
Li, P., Yu, X., Ge, K., Melamed, J., Roeder, R. G., Wang, Z. (2002). Heterogeneous Expression and Functions of Androgen Receptor Co-Factors in Primary Prostate Cancer. Am. J. Pathol. 161: 1467-1474 [Abstract] [Full Text]
Verrijdt, G., Schauwaers, K., Haelens, A., Rombauts, W., Claessens, F. (2002). Functional Interplay between Two Response Elements with Distinct Binding Characteristics Dictates Androgen Specificity of the Mouse Sex-limited Protein Enhancer. J. Biol. Chem. 277: 35191-35201 [Abstract] [Full Text]
Zhao, Y., Goto, K., Saitoh, M., Yanase, T., Nomura, M., Okabe, T., Takayanagi, R., Nawata, H. (2002). Activation Function-1 Domain of Androgen Receptor Contributes to the Interaction between Subnuclear Splicing Factor Compartment and Nuclear Receptor Compartment. IDENTIFICATION OF THE p102 U5 SMALL NUCLEAR RIBONUCLEOPROTEIN PARTICLE-BINDING PROTEIN AS A COACTIVATOR FOR THE RECEPTOR. J. Biol. Chem. 277: 30031-30039 [Abstract] [Full Text]
Wardell, S. E., Boonyaratanakornkit, V., Adelman, J. S., Aronheim, A., Edwards, D. P. (2002). Jun Dimerization Protein 2 Functions as a Progesterone Receptor N-Terminal Domain Coactivator. Mol. Cell. Biol. 22: 5451-5466 [Abstract] [Full Text]
Masiello, D., Cheng, S., Bubley, G. J., Lu, M. L., Balk, S. P. (2002). Bicalutamide Functions as an Androgen Receptor Antagonist by Assembly of a Transcriptionally Inactive Receptor. J. Biol. Chem. 277: 26321-26326 [Abstract] [Full Text]
He, B., Lee, L. W., Minges, J. T., Wilson, E. M. (2002). Dependence of Selective Gene Activation on the Androgen Receptor NH2- and COOH-terminal Interaction. J. Biol. Chem. 277: 25631-25639 [Abstract] [Full Text]
Cheng, S., Brzostek, S., Lee, S. R., Hollenberg, A. N., Balk, S. P. (2002). Inhibition of the Dihydrotestosterone-Activated Androgen Receptor by Nuclear Receptor Corepressor. Mol. Endocrinol. 16: 1492-1501 [Abstract] [Full Text]
Gelmann, E. P. (2002). Molecular Biology of the Androgen Receptor. JCO 20: 3001-3015 [Abstract] [Full Text]
Reid, J., Kelly, S. M., Watt, K., Price, N. C., McEwan, I. J. (2002). Conformational Analysis of the Androgen Receptor Amino-terminal Domain Involved in Transactivation. INFLUENCE OF STRUCTURE-STABILIZING SOLUTES AND PROTEIN-PROTEIN INTERACTIONS. J. Biol. Chem. 277: 20079-20086 [Abstract] [Full Text]
Fu, M., Wang, C., Wang, J., Zhang, X., Sakamaki, T., Yeung, Y. G., Chang, C., Hopp, T., Fuqua, S. A. W., Jaffray, E., Hay, R. T., Palvimo, J. J., Janne, O. A., Pestell, R. G. (2002). Androgen Receptor Acetylation Governs trans Activation and MEKK1-Induced Apoptosis without Affecting In Vitro Sumoylation and trans-Repression Function. Mol. Cell. Biol. 22: 3373-3388 [Abstract] [Full Text]
Tan, J.-A., Hall, S. H., Hamil, K. G., Grossman, G., Petrusz, P., French, F. S. (2002). Protein Inhibitors of Activated STAT Resemble Scaffold Attachment Factors and Function as Interacting Nuclear Receptor Coregulators. J. Biol. Chem. 277: 16993-17001 [Abstract] [Full Text]
Huang, Z.-Q., Li, J., Wong, J. (2002). AR Possesses an Intrinsic Hormone-Independent Transcriptional Activity. Mol. Endocrinol. 16: 924-937 [Abstract] [Full Text]
Kaul, S., Blackford, J. A. Jr., Cho, S., Simons, S. S. Jr. (2002). Ubc9 Is a Novel Modulator of the Induction Properties of Glucocorticoid Receptors. J. Biol. Chem. 277: 12541-12549 [Abstract] [Full Text]
Heinlein, C. A., Chang, C. (2002). Androgen Receptor (AR) Coregulators: An Overview. Endocr. Rev. 23: 175-200 [Abstract] [Full Text]
Dotzlaw, H., Moehren, U., Mink, S., Cato, A. C. B., Iniguez Lluhi, J. A., Baniahmad, A. (2002). The Amino Terminus of the Human AR Is Target for Corepressor Action and Antihormone Agonism. Mol. Endocrinol. 16: 661-673 [Abstract] [Full Text]
Saitoh, M., Takayanagi, R., Goto, K., Fukamizu, A., Tomura, A., Yanase, T., Nawata, H. (2002). The Presence of Both the Amino- and Carboxyl-Terminal Domains in the AR Is Essential for the Completion of a Transcriptionally Active Form with Coactivators and Intranuclear Compartmentalization Common to the Steroid Hormone Receptors: A Three-Dimensional Imaging Study. Mol. Endocrinol. 16: 694-706 [Abstract] [Full Text]
Zhou, Z.-x., He, B., Hall, S. H., Wilson, E. M., French, F. S. (2002). Domain Interactions between Coregulator ARA70 and the Androgen Receptor (AR). Mol. Endocrinol. 16: 287-300 [Abstract] [Full Text]
Markus, S. M., Taneja, S. S., Logan, S. K., Li, W., Ha, S., Hittelman, A. B., Rogatsky, I., Garabedian, M. J. (2002). Identification and Characterization of ART-27, a Novel Coactivator for the Androgen Receptor N Terminus. Mol. Biol. Cell 13: 670-682 [Abstract] [Full Text]
Lee, S. R., Ramos, S. M., Ko, A., Masiello, D., Swanson, K. D., Lu, M. L., Balk, S. P. (2002). AR and ER Interaction with a p21-Activated Kinase (PAK6). Mol. Endocrinol. 16: 85-99 [Abstract] [Full Text]
Gaughan, L., Brady, M. E., Cook, S., Neal, D. E., Robson, C. N. (2001). Tip60 Is a Co-activator Specific for Class I Nuclear Hormone Receptors. J. Biol. Chem. 276: 46841-46848 [Abstract] [Full Text]
Warnmark, A., Wikstrom, A., Wright, A. P. H., Gustafsson, J.-A., Hard, T. (2001). The N-terminal Regions of Estrogen Receptor alpha and beta Are Unstructured in Vitro and Show Different TBP Binding Properties. J. Biol. Chem. 276: 45939-45944 [Abstract] [Full Text]
Yuan, X., Lu, M. L., Li, T., Balk, S. P. (2001). SRY Interacts with and Negatively Regulates Androgen Receptor Transcriptional Activity. J. Biol. Chem. 276: 46647-46654 [Abstract] [Full Text]
Grossmann, M. E., Huang, H., Tindall, D. J. (2001). Androgen Receptor Signaling in Androgen-Refractory Prostate Cancer. JNCI J Natl Cancer Inst 93: 1687-1697 [Abstract] [Full Text]
He, B., Bowen, N. T., Minges, J. T., Wilson, E. M. (2001). Androgen-induced NH2- and COOH-terminal Interaction Inhibits p160 Coactivator Recruitment by Activation Function 2. J. Biol. Chem. 276: 42293-42301 [Abstract] [Full Text]
Shenk, J. L., Fisher, C. J., Chen, S.-Y., Zhou, X.-F., Tillman, K., Shemshedini, L. (2001). p53 Represses Androgen-induced Transactivation of Prostate-specific Antigen by Disrupting hAR Amino- to Carboxyl-terminal Interaction. J. Biol. Chem. 276: 38472-38479 [Abstract] [Full Text]
Dey, R., Roychowdhury, P., Mukherjee, C. (2001). Homology modelling of the ligand-binding domain of glucocorticoid receptor: binding site interactions with cortisol and corticosterone. Protein Eng Des Sel 14: 565-571 [Abstract] [Full Text]
Yang, Z., Privalsky, M. L. (2001). Isoform-Specific Transcriptional Regulation by Thyroid Hormone Receptors: Hormone-Independent Activation Operates through a Steroid Receptor Mode of Coactivator Interaction. Mol. Endocrinol. 15: 1170-1185 [Abstract] [Full Text]
Aranda, A., Pascual, A. (2001). Nuclear Hormone Receptors and Gene Expression. Physiol. Rev. 81: 1269-1304 [Abstract] [Full Text]
Thompson, J., Saatcioglu, F., Janne, O. A., Palvimo, J. J. (2001). Disrupted Amino- and Carboxyl-Terminal Interactions of the Androgen Receptor Are Linked to Androgen Insensitivity. Mol. Endocrinol. 15: 923-935 [Abstract] [Full Text]
Grad, J. M., Lyons, L. S., Robins, D. M., Burnstein, K. L. (2001). The Androgen Receptor (AR) Amino-Terminus Imposes Androgen-Specific Regulation of AR Gene Expression via an Exonic Enhancer. Endocrinology 142: 1107-1116 [Abstract] [Full Text]
Kotaja, N., Aittomäki, S., Silvennoinen, O., Palvimo, J. J., Jänne, O. A. (2000). ARIP3 (Androgen Receptor-Interacting Protein 3) and Other PIAS (Protein Inhibitor of Activated STAT) Proteins Differ in Their Ability to Modulate Steroid Receptor-Dependent Transcriptional Activation. Mol. Endocrinol. 14: 1986-2000 [Abstract] [Full Text]
Ren, Y., Behre, E., Ren, Z., Zhang, J., Wang, Q., Fondell, J. D. (2000). Specific Structural Motifs Determine TRAP220 Interactions with Nuclear Hormone Receptors. Mol. Cell. Biol. 20: 5433-5446 [Abstract] [Full Text]
Lim, J., Ghadessy, F. J., Abdullah, A. A. R., Pinsky, L., Trifiro, M., Yong, E. L. (2000). Human Androgen Receptor Mutation Disrupts Ternary Interactions between Ligand, Receptor Domains, and the Coactivator TIF2 (Transcription Intermediary Factor 2). Mol. Endocrinol. 14: 1187-1197 [Abstract] [Full Text]
Schoenmakers, E., Verrijdt, G., Peeters, B., Verhoeven, G., Rombauts, W., Claessens, F. (2000). Differences in DNA Binding Characteristics of the Androgen and Glucocorticoid Receptors Can Determine Hormone-specific Responses. J. Biol. Chem. 275: 12290-12297 [Abstract] [Full Text]
Verrijdt, G., Schoenmakers, E., Haelens, A., Peeters, B., Verhoeven, G., Rombauts, W., Claessens, F. (2000). Change of Specificity Mutations in Androgen-selective Enhancers. EVIDENCE FOR A ROLE OF DIFFERENTIAL DNA BINDING BY THE ANDROGEN RECEPTOR. J. Biol. Chem. 275: 12298-12305 [Abstract] [Full Text]
He, B., Kemppainen, J. A., Wilson, E. M. (2000). FXXLF and WXXLF Sequences Mediate the NH2-terminal Interaction with the Ligand Binding Domain of the Androgen Receptor. J. Biol. Chem. 275: 22986-22994 [Abstract] [Full Text]
Gonzalez, M. I., Robins, D. M. (2001). Oct-1 Preferentially Interacts with Androgen Receptor in a DNA-dependent Manner That Facilitates Recruitment of SRC-1. J. Biol. Chem. 276: 6420-6428 [Abstract] [Full Text]
Wang, Q., Lu, J., Yong, E. L. (2001). Ligand- and Coactivator-mediated Transactivation Function (AF2) of the Androgen Receptor Ligand-binding Domain Is Inhibited by the Cognate Hinge Region. J. Biol. Chem. 276: 7493-7499 [Abstract] [Full Text]
Song, L.-N., Huse, B., Rusconi, S., Simons, S. S. Jr. (2001). Transactivation Specificity of Glucocorticoid Versus Progesterone Receptors. ROLE OF FUNCTIONALLY DIFFERENT INTERACTIONS OF TRANSCRIPTION FACTORS WITH AMINO- AND CARBOXYL-TERMINAL RECEPTOR DOMAINS. J. Biol. Chem. 276: 24806-24816 [Abstract] [Full Text]
Slagsvold, T., Kraus, I., Fronsdal, K., Saatcioglu, F. (2001). DNA Binding-independent Transcriptional Activation by the Androgen Receptor through Triggering of Coactivators. J. Biol. Chem. 276: 31030-31036 [Abstract] [Full Text]
Bubulya, A., Chen, S.-Y., Fisher, C. J., Zheng, Z., Shen, X.-Q., Shemshedini, L. (2001). c-Jun Potentiates the Functional Interaction between the Amino and Carboxyl Termini of the Androgen Receptor. J. Biol. Chem. 276: 44704-44711 [Abstract] [Full Text]
Ting, H.-J., Yeh, S., Nishimura, K., Chang, C. (2002). Supervillin associates with androgen receptor and modulates its transcriptional activity. Proc. Natl. Acad. Sci. USA 99: 661-666 [Abstract] [Full Text]

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1.	Aarnisalo, P., J. J. Palvimo, and O. A. Jänne. 1998. CREB-binding protein in androgen receptor-mediated signaling. Proc. Natl. Acad. Sci. USA 95:2122-2127[Abstract/Free Full Text].
2.	Alen, P., F. Claessens, E. Schoenmakers, J. V. Swinnen, G. Verhoeven, W. Rombauts, and B. Peeters. 1999. Interaction of the putative androgen receptor-specific coactivator ARA₇₀/ELE1 $alpha$ with multiple steroid receptors and identification of an internally deleted ELE1 $beta$ isoform. Mol. Endocrinol. 13:117-128[Abstract/Free Full Text].
3.	Anzick, S. L., J. Kononen, R. L. Walker, D. O. Azorsa, M. M. Tanner, X. Y. Guan, G. Sauter, O. P. Kallioniemi, J. M. Trent, and P. S. Meltzer. 1997. AIB1, a steroid receptor coactivator amplified in breast and ovarian cancer. Science 277:965-968[Abstract/Free Full Text].
4.	Baniahmad, A., A. C. Kohne, and R. Renkawitz. 1992. A transferable silencing domain is present in the thyroid hormone receptor, in the v-erbA oncogene product and in the retinoic acid receptor. EMBO J. 11:1015-1023[Medline].
5.	Bannister, A. J., and T. Kouzarides. 1996. The CBP co-activator is a histone acetyltransferase. Nature 384:641-643[Medline].
6.	Beato, M., S. Chavez, and M. Truss. 1996. Transcriptional regulation by steroid hormones. Steroids 61:240-251[Medline].
7.	Beato, M., and A. Sanchez-Pacheco. 1996. Interaction of steroid hormone receptors with the transcription initiation complex. Endocrine Rev. 17:587-609[Abstract/Free Full Text].
8.	Berrevoets, C. A., P. Doesburg, K. Steketee, J. Trapman, and A. O. Brinkmann. 1998. Functional interactions of the AF-2 activation domain core region of the human androgen receptor with the amino-terminal domain and with the transcriptional coactivator TIF2 (transcriptional intermediary factor 2). Mol. Endocrinol. 12:1172-1183[Abstract/Free Full Text].
9.	Blanco, J. C. G., S. Minucci, J. Lu, X. J. Yang, K. K. Walker, H. Chen, R. M. Evans, Y. Nakatani, and K. Ozato. 1998. The histone acetylase PCAF is a nuclear receptor coactivator. Genes Dev. 12:1638-1651[Abstract/Free Full Text].
10.	Buchert, M., S. Schneider, M. T. Adams, H. P. Hefti, K. Moelling, and C. M. Hovens. 1997. Useful vectors for the two-hybrid system in mammalian cells. BioTechniques 23:396-402[Medline].
11.	Chamberlain, N. L., D. C. Whitacre, and R. L. Miesfeld. 1996. Delineation of two distinct type 1 activation functions in the androgen receptor amino-terminal domain. J. Biol. Chem. 271:26772-26778[Abstract/Free Full Text].
12.	Chen, H., R. J. Lin, R. L. Schiltz, D. Chakravarti, A. Nash, L. Nagy, M. L. Privalsky, Y. Nakatani, and R. Evans. 1997. Nuclear receptor coactivator ACTR is a novel histone acetyltransferase and forms a multimeric activation complex with P/CAF and CBP/p300. Cell 90:569-580[Medline].
13.	Danielian, P. S., R. White, J. A. Lees, and M. G. Parker. 1992. Identification of a conserved region required for hormone dependent transcriptional activation by steroid hormone receptors. EMBO J. 11:1025-1033[Medline].
14.	Ding, X. F., C. M. Anderson, H. Ma, H. Hong, R. M. Uht, P. Kushner, and M. R. Stallcup. 1998. Nuclear receptor-binding sites of coactivators glucocorticoid receptor interaction protein 1(GRIP1) and steroid receptor coactivator 1 (SRC1): multiple motifs with different binding specificities. Mol. Endocrinol. 12:302-313[Abstract/Free Full Text].
15.	Doesburg, P., C. W. Kuil, C. A. Berrevoets, K. Steketee, P. W. Faber, E. Mulder, A. O. Brinkmann, and J. Trapman. 1997. Functional in vivo interaction between the amino-terminal and the ligand binding domain of the androgen receptor. Biochemistry 36:1052-1064[Medline].
16.	Fawell, S. E., J. A. Lees, R. White, and M. G. Parker. 1990. Characterization and colocalization of steroid binding and dimerization activities in the mouse estrogen receptor. Cell 60:953-962[Medline].
17.	Feng, W., R. C. J. Ribeiro, R. L. Wagner, H. Nguyen, J. W. Apriletti, R. J. Fletterick, J. D. Baxter, P. J. Kushner, and B. L. West. 1998. Hormone-dependent coactivator binding to a hydrophobic cleft on nuclear receptors. Science 280:1747-1749[Abstract/Free Full Text].
18.	Fronsdal, K., N. Engedal, T. Slagsvold, and F. Saatcioglu. 1998. CREB binding protein is a coactivator for the androgen receptor and mediates cross-talk with AP-1. J. Biol. Chem. 273:31853-31859[Abstract/Free Full Text].
19.	Heery, D. M., E. Kalkhoven, S. Hoare, and M. G. Parker. 1997. A signature motif in transcriptional co-activators mediates binding to nuclear receptors. Nature 387:733-736[Medline].
20.	Henttu, P. M. A., E. Kalkhoven, and M. G. Parker. 1997. AF-2 activity and recruitment of steroid receptor coactivator 1 to the estrogen receptor depend on a lysine residue conserved in nuclear receptors. Mol. Cell. Biol. 17:1832-1839[Abstract].
21.	Hong, H., K. Kohli, M. J. Garabedian, and M. R. Stallcup. 1997. GRIP1, a transcriptional coactivator for the AF-2 transactivation domain of steroid, thyroid, retinoid, and vitamin D receptors. Mol. Cell. Biol. 17:2735-2744[Abstract].
22.	Hong, H., B. D. Darimont, H. Ma, L. Yang, K. R. Yamamoto, and M. R. Stallcup. 1999. An additional region of coactivator GRIP1 required for interaction with the hormone-binding domains of a subset of nuclear receptors. J. Biol. Chem. 274:3496-3502[Abstract/Free Full Text].
23.	Horwitz, K. B., T. A. Jackson, D. L. Bain, J. K. Richer, G. S. Takimoto, and L. Tung. 1996. Nuclear receptor coactivators and corepressors. Mol. Endocrinol. 10:1167-1177[Abstract/Free Full Text].
24.	Ikonen, T., J. J. Palvimo, and O. A. Jänne. 1997. Interaction between the amino- and carboxyl-terminal regions of the rat androgen receptor modulates transcriptional activity and is influenced by nuclear receptor coactivators. J. Biol. Chem. 272:29821-29828[Abstract/Free Full Text].
25.	Jenster, G., H. A. G. M. van der Korput, C. C. J. van Groonhoven, T. H. Van der Kwast, J. Trapman, and A. O. Brinkmann. 1991. Domains of the human androgen receptor involved in steroid binding, transcriptional activation, and subcellular localization. Mol. Endocrinol. 5:1396-1404[Abstract/Free Full Text].
26.	Jenster, G., H. A. G. M. van der Korput, J. Trapman, and A. O. Brinkmann. 1995. Identification of two transcription activation units in the N-terminal domain of the human androgen receptor. J. Biol. Chem. 270:7341-7346[Abstract/Free Full Text].
27.	Jenster, G. 1998. Coactivators and corepressors as mediators of nuclear receptor function: an update. Mol. Cell. Endocrinol. 143:1-7[Medline].
28.	Jeyakumar, M., M. R. Tanen, and M. K. Bagchi. 1997. Analysis of the functional role of steroid receptor coactivator-1 in ligand-induced transactivation by thyroid hormone receptor. Mol. Endocrinol. 11:755-767[Abstract/Free Full Text].
29.	Kalkhoven, E., J. E. Valentin, D. M. Heery, and M. G. Parker. 1998. Isoforms of steroid receptor co-activator 1 differ in their ability to potentiate transcription by the oestrogen receptor. EMBO J. 17:232-243[Medline].
30.	Kamei, Y., L. Xu, T. Heinzel, J. Torchia, R. Kurokawa, B. Gloss, S.-C. Lin, R. A. Heyman, D. W. Rose, C. K. Glass, and M. G. Rosenfeld. 1996. A CBP integrator complex mediates transcriptional activation and AP-1 inhibition by nuclear receptors. Cell 85:403-414[Medline].
31.	Langley, E., Z. X. Zhou, and E. M. Wilson. 1995. Evidence for an anti-parallel orientation of the ligand-activated human androgen receptor dimer. J. Biol. Chem. 270:29983-29990[Abstract/Free Full Text].
32.	Langley, E., J. A. Kemppainen, and E. M. Wilson. 1998. Intermolecular NH₂-carboxyl-terminal interactions in androgen receptor dimerization revealed by mutations that cause androgen insensitivity. J. Biol. Chem. 273:92-101[Abstract/Free Full Text].
33.	Lavinsky, R. M., K. Jepsen, T. Heinzel, J. Torchia, T.-M. Mullen, R. Schiff, A. L. Del-Rio, M. Ricolte, S. Ngo, J. Gemsch, S. G. Hilsenbeck, C. K. Osborne, C. K. Glass, M. G. Rosenfeld, and D. W. Rose. 1998. Diverse signaling pathways modulate nuclear receptor recruitment of N-CoR and SMRT complexes. Proc. Natl. Acad. Sci. USA 95:2920-2925[Abstract/Free Full Text].
34.	Leers, J., E. Treuter, and J. A. Gustaffson. 1998. Mechanistic principles in NR box-dependent interaction between nuclear hormone receptors and the coactivator TIF2. Mol. Cell. Biol. 18:6001-6013[Abstract/Free Full Text].
35.	Li, H., P. J. Gomes, and D. J. Chen. 1996. RAC3, a steroid/nuclear receptor-associated coactivator that is related to SRC-1 and TIF2. Proc. Natl. Acad. Sci. USA 94:8479-8484[Abstract/Free Full Text].
36.	Li, H., and D. Chen. 1998. The receptor-associated coactivator 3 activates transcription through CREB-binding protein recruitment and autoregulation. J. Biol. Chem. 273:5948-5954[Abstract/Free Full Text].
37.	Mangelsdorf, D. J., C. Thummel, M. Beato, P. Herrlich, G. Schutz, K. Umesono, B. Blumberg, P. Kastner, M. Mark, P. Chambon, and R. Evans. 1995. The nuclear receptor superfamily: the second decade. Cell 83:835-839[Medline].
38.	Marivoet, S., M. Hertogen, G. Verhoeven, and W. Heyns. 1990. Antibodies against synthetic peptide recognise the human and rat androgen receptor. J. Steroid Biochem. Mol. Biol. 37:39-45[Medline].
39.	McInerney, E. M., M. J. Tsai, B. W. O'Malley, and B. S. Katzenellenbogen. 1996. Analysis of estrogen receptor transcriptional enhancement by a nuclear hormone receptor coactivator. Proc. Natl. Acad. Sci. USA 93:10069-10073[Abstract/Free Full Text].
40.	Moilanen, A., N. Rouleau, T. Ikonen, J. J. Palvimo, and O. A. Jänne. 1997. The presence of a transcription activation function in the hormone-binding domain of androgen receptor is revealed by studies in yeast cells. FEBS Lett. 412:355-358[Medline].
41.	Moilanen, A., H. Poukka, U. Karvonen, M. Häkli, O. A. Jänne, and J. J. Palvimo. 1998. Identification of a novel RING finger protein as a coregulator in steroid receptor-mediated gene transcription. Mol. Cell. Biol. 18:5128-5139[Abstract/Free Full Text].
42.	Moras, D., and H. Gronemeyer. 1998. The nuclear receptor ligand-binding domain: structure and function. Curr. Opin. Cell Biol. 10:384-391[Medline].
43.	Nolte, R. T., G. B. Wisely, S. Westin, J. E. Cobb, M. Lambert, R. Kurokawa, M. Rosenfeld, T. M. Willson, C. K. Glass, and M. V. Milburn. 1998. Ligand binding and co-activator assembly of the peroxisome proliferator-activated receptor- $gamma$ . Nature 395:137-143[Medline].
44.	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[Medline].
45.	Onate, S. A., S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1995. Sequence and characterization of a coactivator for the steroid hormone receptor superfamily. Science 270:1354-1357[Abstract/Free Full Text].
46.	Onate, S. A., V. Boonyaratanakornkit, T. E. Spencer, S. Y. Tsai, M. J. Tsai, D. P. Edwards, and B. W. O'Malley. 1998. The steroid receptor coactivator-1 contains multiple receptor interaction domains that cooperatively enhance the activation function 1 (AF1) and AF2 domains of steroid receptors. J. Biol. Chem. 273:12101-12108[Abstract/Free Full Text].
47.	Parker, M. G., and R. White. 1996. Nuclear receptors spring into action. Nat. Struct. Biol. 3:113-115[Medline].
48.	Plaisance, S., W. VandenBerghe, E. Boone, W. Fiers, and G. Haegeman. 1997. Recombination signal sequence binding protein J kappa is constitutively bound to the NF-kappa B site of the interleukin-6 promoter and acts as a negative regulatory factor. Mol. Cell. Biol. 17:3733-3743[Abstract].
49.	Quigley, C. A., A. De Bellis, K. B. Marschke, M. K. El-Awady, E. M. Wilson, and F. S. French. 1995. Androgen receptor defects: historical, clinical, and molecular perspectives. Endocrine Rev. 16:271-321[Abstract/Free Full Text].
50.	Schmidt, S., A. Baniahmad, M. Eggert, S. Schneider, and R. Renkawitz. 1998. Multiple receptor interaction domains of GRIP1 function in synergy. Nucleic Acids. Res. 26:1191-1197[Abstract/Free Full Text].
51.	Shiau, A. K., D. Barstad, P. M. Loria, L. Cheng, P. J. Kushner, D. A. Agard, and G. L. Greene. 1999. The structural basis of estrogen receptor/coactivator recognition and the antagonism of this interaction by tamoxifen. Cell 95:927-937.
52.	Shibata, H., T. E. Spencer, S. A. Onate, G. Jenster, S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1997. Role of coactivators and corepressors in the mechanism of steroid/thyroid receptor action. Recent Prog. Horm. Res. 52:141-165.
53.	Simental, J. A., M. Sar, and E. M. Wilson. 1992. Domain functions of the androgen receptor. J. Steroid Biochem. Mol. Biol. 43:37-41[Medline].
54.	Smith, C. L., Z. Nawaz, and B. W. O'Malley. 1997. Coactivator and corepressor regulation of the agonist/antagonist activity of the mixed antiestrogen, 4-hydroxytamoxifen. Mol. Endocrinol. 11:657-666[Abstract/Free Full Text].
55.	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[Medline].
56.	Suen, C. S., T. J. Berrodin, R. Mastroeni, B. J. Cheskis, C. R. Lyttle, and D. E. Frail. 1998. A transcriptional coactivator, steroid receptor coactivator-3, selectively augments steroid receptor transcriptional activity. J. Biol. Chem. 273:27645-27653[Abstract/Free Full Text].
57.	Takeshita, A., P. M. Yen, S. Misti, G. R. Cardona, Y. Liu, and W. W. Chin. 1996. Molecular cloning and properties of a full-length putative thyroid hormone receptor coactivator. Endocrinology 137:3594-3597[Abstract].
58.	Takeshita, A., G. R. Cardona, N. Koibuchi, C. S. Suen, and W. W. Chin. 1997. TRAM-1, a novel 160-kDa thyroid hormone receptor activator molecule, exhibits distinct properties from steroid receptor coactivator-1. J. Biol. Chem. 272:27629-27634[Abstract/Free Full Text].
59.	Takeshita, A., P. M. Yen, M. Ikeda, G. R. Cardona, Y. Liu, N. Koibuchi, E. R. Norwitz, and W. W. Chin. 1998. Thyroid hormone response elements differentially modulate the interactions of thyroid hormone receptors with two receptor binding domains in the steroid receptor coactivator-1. J. Biol. Chem. 273:21554-21562[Abstract/Free Full Text].
60.	Torchia, J., D. W. Rose, J. Inostroza, Y. Kamei, S. Westin, C. Glass, and M. G. Rosenfeld. 1997. The transcriptional co-activator p/CIP binds CBP and mediates nuclear-receptor function. Nature 387:677-684[Medline].
61.	Torchia, J., C. Glass, and M. Rosenfeld. 1998. Co-activators and co-repressors in the integration of transcriptional responses. Curr. Opin. Cell. Biol. 10:373-383[Medline].
62.	Tsai, M. J., and B. W. O'Malley. 1994. Molecular mechanisms of action of steroid/thyroid receptor superfamily members. Annu. Rev. Biochem. 63:451-486[Medline].
63.	Tsai, R. Y. L., and R. R. Reed. 1997. Using a eukaryotic GST fusion vector for proteins difficult to express in E. coli. BioTechniques 23:794-800[Medline].
64.	Voegel, J. J., M. J. S. Heine, C. Zechel, P. Chambon, and H. Gronemeyer. 1996. TIF2, a 160 kDa transcriptional mediator for the ligand-dependent activation function AF-2 of nuclear receptors. EMBO J. 15:3667-3675[Medline].
65.	Voegel, J. J., M. J. S. Heine, M. Tini, V. Vivat, P. Chambon, and H. Gronemeyer. 1998. The coactivator TIF2 contains three nuclear receptor-binding motifs and mediates transactivation through CBP binding-dependent and -independent pathways. EMBO J. 17:507-519[Medline].
66.	Webb, P., P. Nguyen, J. Shinsako, C. Anderson, W. Feng, M. P. Nguyen, D. Chen, S. M. Huang, S. Subramanian, E. McKinerney, B. S. Katzenellenbogen, M. R. Stallcup, and P. J. Kushner. 1998. Estrogen receptor activation function 1 works by binding p160 coactivator proteins. Mol. Endocrinol. 12:1605-1618[Abstract/Free Full Text].
67.	Williams, S. P., and P. B. Sigler. 1998. Atomic structure of progesterone complexed with its receptor. Nature 393:392-396[Medline].
68.	Wong, C. I., Z. X. Zhou, M. Sar, and E. M. Wilson. 1993. Steroid requirements for androgen receptor dimerization and DNA binding. J. Biol. Chem. 268:19004-19012[Abstract/Free Full Text].
69.	Wurtz, J. M., W. Bourguet, J. P. Renaud, V. Vivat, P. Chambon, D. Moras, and H. Gronemeyer. 1996. A canonical structure for the ligand-binding domain of nuclear receptors. Nat. Struct. Biol. 3:87-94[Medline].
70.	Xu, J., Z. Nawaz, S. Y. Tsai, M. J. Tsai, and B. W. O'Malley. 1996. The extreme C-terminus of the progesterone receptor contains a transcriptional repressor domain that functions through a putative corepressor. Proc. Natl. Acad. Sci. USA 93:12195-12199[Abstract/Free Full Text].
71.	Yang, X. J., V. V. Ogryzko, J. I. Nishikawa, B. Howard, and Y. Nakatani. 1996. A p300/CBP-associated factor that competes with the adenoviral oncoprotein E1A. Nature 283:319-324.
72.	Zhou, G., R. Cummings, Y. Li, S. Mitra, H. A. Wilkinson, A. Elbrecht, J. D. Hermes, J. M. Schaeffer, R. G. Smith, and D. E. Moller. 1998. Nuclear receptors have distinct affinities for coactivators: characterization by fluorescence resonance energy transfer. Mol. Endocrinol. 12:1594-1604[Abstract/Free Full Text].