Suppression of sterol 12{alpha}-hydroxylase transcription by the short heterodimer partner: insights into the repression mechanism

doi:10.1093/nar/29.19.4035

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Nucleic Acids Research, 2001, Vol. 29, No. 19 4035-4042
© 2001 Oxford University Press

Suppression of sterol 12 ${alpha}$ -hydroxylase transcription by the short heterodimer partner: insights into the repression mechanism

Antonio del Castillo-Olivares and Gregorio Gil^*

Department of Biochemistry and Molecular Biophysics, Medical College of Virginia, PO Box 980614, Richmond, VA 23298-0614, USA

Received May 23, 2001; Revised and Accepted August 16, 2001.

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cholesterol conversion to bile acids is subject to a feedbackregulatory mechanism by which bile acids down-regulate theirown synthesis. This regulation occurs at the level of transcriptionof several genes encoding enzymes in the bile acid biosyntheticpathway. One of these enzymes is sterol 12 ${alpha}$ -hydroxylase/CYP8B1(12 ${alpha}$ -hydroxylase), the specific enzyme required for cholic acidsynthesis. The levels of this enzyme determine the ratio ofcholic acid to chenodeoxycholic acid and thus the hydrophobicityof the circulating bile acid pool. Previous studies from thislaboratory showed that fetoprotein transcription factor (FTF)is required for 12 ${alpha}$ -hydroxylase promoter activity and bile acid-mediatedregulation. Here, we report that the short heterodimer partner(SHP) suppresses 12 ${alpha}$ -hydroxylase promoter activity via an interactionwith FTF. Hepatic nuclear factor-4 (HNF-4) binds and activatesthe 12 ${alpha}$ -hydroxylase promoter and is required for 12 ${alpha}$ -hydroxylasepromoter activity. Although HNF-4 interacts with SHP, it isnot involved in SHP-mediated suppression of 12 ${alpha}$ -hydroxylase promoteractivity. FTF and not HNF-4 is the factor involved in regulationof 12 ${alpha}$ -hydroxylase promoter activity by bile acids through itsinteraction with SHP. Finally, interaction of SHP with FTF displacesFTF binding to its sites within the 12 ${alpha}$ -hydroxylase promoter.These results provide insights into the mechanism of actionof bile acid-mediated regulation of sterol 12 ${alpha}$ -hydroxylase transcription.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Bile acid synthesis plays a crucial role in maintaining cholesterolhomeostasis since it is responsible for the catabolism of >50%of body cholesterol. Bile acids also stimulate the excretionof excess hepatic cholesterol into bile. In the intestine, bileacids play an important role in the solubilization and absorptionof fat-soluble vitamins and cholesterol. Thus, proper controlof bile acid synthesis is important and is achieved throughthe regulation of several enzymes: cholesterol 7 ${alpha}$ -hydroxylase/CYP7A1(7 ${alpha}$ -hydroxylase), the rate-limiting enzyme in the classic pathway(1); sterol 27-hydroxylase/CYP27, the first enzyme in thealternative pathway (2); and sterol 12 ${alpha}$ -hydroxylase/CYP8B1 (12 ${alpha}$ -hydroxylase),the specific enzyme for cholic acid synthesis that determinesthe ratio of cholic acid to chenodeoxycholic acid (CDCA) andthus the hydrophobicity of the circulating pool (3).

Bile acids negatively regulate transcription of the 7 ${alpha}$ -hydroxylasegene, which controls output from the classic pathway. Recentstudies have delineated many of the factors involved in thisregulation. Liver receptor homolog-1, also known as CYP7A promoter-bindingfactor (CPF), NR5A2 (4) and fetoprotein transcription factor(FTF) (Genome Database Nomenclature Committee) (5) have beenproposed to be required for transcription of the 7 ${alpha}$ -hydroxylasegene (6). Bile acids activate transcription of the small heterodimerpartner 1 (SHP) via binding of the hormone receptor farnesilX receptor (FXR) to its binding site in the SHP promoter. Inturn, it has been proposed that SHP dimerizes with FTF and diminishesits activity on the 7 ${alpha}$ -hydroxylase promoter by mechanisms notyet well understood (7,8). An alternative mechanism has recentlybeen proposed for this down-regulation of 7 ${alpha}$ -hydroxylase transcriptionthat involves the c-Jun N-terminal kinase (JNK) (9). In thismechanism, the JNK pathway is activated by bile acids, whichin turns activates c-Jun resulting in higher SHP transcription.

SHP is an orphan nuclear receptor originally identified onthe basis of its interaction with the receptor CAR (10). Itlacks a DNA-binding domain and interacts with several receptors,among them hepatic nuclear receptor-4 (HNF-4) (11), estrogenreceptor (ER) (12) and retinoid X receptor ${alpha}$ (RXR) (10). Uponinteraction with these receptors, SHP acts to decrease transactivationby its partners in transient transfection assays. This inhibitoryeffect was first attributed to an inhibition of DNA bindingby the SHP targets (10). Further studies, however, revealedthat SHP carries a repression domain in its C-terminal domain(13) suggesting that SHP could inhibit transcription withoutinterference with binding of its partner to the DNA. This alternativemechanism was confirmed by the demonstration that SHP is aninhibitor of ER transactivation, even though it does not preventbinding of ER to estrogen response elements (13).

Another enzyme in the bile acid biosynthetic pathway that isalso regulated by bile acids is 12 ${alpha}$ -hydroxylase (3,14,15). Wehave recently shown that FTF is required for 12 ${alpha}$ -hydroxylasepromoter activity (16). FTF binds to two sites within the 12 ${alpha}$ -hydroxylasepromoter and both sites are required for both promoter activityand bile acid-mediated regulation. However, it has not beenshown whether SHP is involved in this regulation, much lessthe mechanisms by which SHP suppresses FTF activity on bileacid regulated genes.

The two FTF sites in the 12 ${alpha}$ -hydroxylase promoter overlap witha direct repeat (DR-1) element that binds peroxisome proliferator-activatedreceptor ${alpha}$ (PPAR ${alpha}$ ) and mediates peroxisome proliferator activationof 12 ${alpha}$ -hydroxylase transcription (17). Interestingly, the 7 ${alpha}$ -hydroxylasepromoter also contains a DR-1 element, which is a binding sitefor HNF-4 among other nuclear receptors. It has been shown thatHNF-4 indeed does bind and activate the 7 ${alpha}$ -hydroxylase promoter(18). The existence of HNF-4 sites overlapping the FTF sitesin both the 7 ${alpha}$ -hydroxylase and 12 ${alpha}$ -hydroxylase promoters togetherwith the fact that SHP is a repressor of HNF-4 (11) raises thepossibility that HNF-4 is involved in bile acid regulation ofgene transcription through its interaction with SHP.

In this study we show that SHP is involved in down-regulationof the 12 ${alpha}$ -hydroxylase promoter. Overexpression of SHP in HepG2cells suppresses 12 ${alpha}$ -hydroxylase promoter activity. We also showthat HNF-4 is required for 12 ${alpha}$ -hydroxylase promoter activity,but despite the interaction between HNF-4 and SHP, bile acidsonly suppress FTF-activated 12 ${alpha}$ -hydroxylase promoters. Additionally,we show that several SHP domains are required for that interaction,suggesting a complex mode of contact between FTF and SHP. Finally,we show that SHP prevents binding of FTF to its bindingsites within the 12 ${alpha}$ -hydroxylase promoter, providing a mechanismof action for SHP-mediated suppression of 12 ${alpha}$ -hydroxylase transcription.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials
Reagents used in DNA cloning and sequencing were from New EnglandBiolabs, Boehringer Mannheim, US Biochemical Corp. and GibcoBRL. Common laboratory chemicals were from Fisher, Sigma orBio-Rad. Oligonucleotides were prepared in the Medical Collegeof Virginia DNA Synthesis Facility by the phosphoramidite methodon an automated DNA synthesizer. The luciferase promoter-lessvector, pGL3-Basic, was purchased from Promega. The mammaliantwo-hybrid vectors pVP16 and pM were purchased from Clontech.pCMX, a plasmid for expression in mammalian cells and in vitro,contains the CMV and T7 promoters, and TK-MH100x4-LUC, a plasmidthat has four copies of the Gal4 DNA-binding domain in frontof the luciferase reporter gene, were a gift from Dr RonaldM. Evans (The Salk Institute, La Jolla, CA). pCI/hFTF, an expressionplasmid that contains the human FTF cDNA in the expression vectorpCI (Promega), pCI/hFTF ${Delta}$ LBD and pCI/hFTF ${Delta}$ AF2 were a generous giftfrom Dr Bélanger (L’University Laval, Quebec, Canada).pCDM8/mSHP, an expression plasmid containing full-length mouseSHP, and all the other SHP plasmids used in this study wereobtained from Dr Moore (Baylor College of Medicine, Houston,TX). pGL3-R12 ${alpha}$ -865 is a promoter reporter construct that contains865 bp of the rat 12 ${alpha}$ -hydroxylase promoter in the pGL3 vector(16). The three 12 ${alpha}$ -hydroxylase promoter constructs used forthe experiments shown in Figure 3A were made using a QuickChangesite-directed mutagenesis kit (Stratagene) and the correspondingoligonucleotides. pGHR contains the rabbit growth hormone receptorcDNA in pCMV (19,20). Anti-HNF-4 antibodies were obtained fromSanta Cruz Biotechnology Inc. and anti-FTF antibodies were agift from Dr David W. Russell (Southwestern Medical Center,Dallas, TX) and were raised against a peptide correspondingto amino acids 180–197 of the DNA-binding domain.

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Figure 3. The 12 ${alpha}$ -hydroxylase DR-1 HNF-4-binding site is required for 12 ${alpha}$ -hydroxylase promoter activity. (A) Three 12 ${alpha}$ -hydroxylase promoter mutants were created as shown, with the mutated nucleotides in small capital letters. FTF sites are indicated by slashed boxes and the hexamers corresponding to the DR-1 site are shown by arrows. The wild-type 12 ${alpha}$ -hydroxylase promoter construct and the three mutants were transfected into HepG2 cells, incubated in the absence or presence of CDCA and relative promoter activity quantified as indicated in Materials and Methods. Data represent the means ± SD of four assays performed in duplicate. ND, not detectable (activity was $<=$ 1.5-fold that obtained with the empty vector pGL3, whereas the wild-type 12 ${alpha}$ -hydroxylase promoter had 80-fold higher activity than pGL3). (B) Gel shift experiments were performed using the indicated probes and either in vitro synthesized FTF or HNF-4 proteins or in vitro produced GHR as a control. Arrows point to the retarded bands as well as the free probes.

General methods
Standard recombinant DNA procedures were carried out essentiallyas described (16).

Preparation of chimeric FTF expression plasmids
pCMX/FTF was prepared by inserting a 1600 nt SacII–SalIfragment from pCI/FTF into the BamHI site of pCMX. The FTF deletionplasmids were prepared by inserting the corresponding fragment,prepared by PCR with specific oligonucleotides, into its correspondingvector. pVP16-FTF was prepared by inserting the FTF cDNA intopVP16 (Clontech). Orientation and correct frame were confirmedby sequencing.

Transient transfection and luciferase assays
HepG2, Hep3B and CV-1 cells were obtained from the AmericanType Culture Collection. HepG2 and Hep3B cells were transfectedby the calcium phosphate method using 2.0 µg total DNA.CV-1 cells were transfected with Lipofectin (Gibco) and 750ng total DNA. HepG2 cells were transfected with 100 ng testplasmid, 5 ng pCMV-Gal [a plasmid containing the human cytomegalovirus(CMV) promoter in front of the bacterial ß-galactosidasegene] to normalize for transfection efficiencies and the indicatedamounts of wild-type pCDM8/mSHP. For SHP overexpression, CV-1cells were transfected with 100 ng test plasmid, 10 ng pCMV-Gal,100 ng pCI-FTF, an expression plasmid containing the FTF cDNAdriven by the CMV promoter, and the indicated amounts of wild-typepCDM8/mSHP or the W160X mutant. For the mammalian two-hybridsystem CV-1 cells were transfected with 100 ng TK-MH100x4-LUC,as a reporter plasmid, 25 ng pCMV-Gal and 325 ng each indicatedhybrid. Hep3B cells were transfected with 250 ng test plasmid,10 ng pCMV-Gal and 750 ng pCI/hFTF or the indicated deletionmutant. After 16 h the DNA was removed and, where indicated,100 µM CDCA was added. Cells were harvested 48 h laterand luciferase and ß-galactosidase assays were performedwith a kit from Tropix (Bedford, MA), according to the manufacturer’sprotocol. Average values are for the number of experiments indicated.

In vitro transcription/translation and HepG2 nuclear extracts
Transcription/translation of cDNAs encoding FTF, SHP or thegrowth hormone receptor (GHR) as a control was performed usingthe TNT T7-coupled rabbit reticulocyte lysate system accordingto the manufacturer’s protocol (Promega). Proteins weresynthesized with [³⁵S]L-methionine and quantified using a MolecularDynamics PhosphorImager. HepG2 nuclear extracts were preparedas indicated (16).

Electrophoretic mobility shift analysis and SDS–PAGE
DNA binding reactions contained 50 mM KCl, 20 mM Tris–HClpH 8.0, 0.2 mM EDTA, 4% Ficoll, 1.0 µg poly(dI–dC),4 µl of the translated protein and a 1500-fold molar excessof an irrelevant single-stranded DNA, in a final volume of 20µl on ice. After 15 min incubation, 32 fmol ³²P-labeledDNA probe ( $~$ 2 x 10⁵ c.p.m.) were added. The probe used containednucleotides –69 to –46 from the 12 ${alpha}$ -hydroxylase promoter.After incubation for 20 min on ice, samples were loaded ontoa 4.5% polyacrylamide gel and subjected to electrophoresis at4°C. Gels were dried and exposed to XAR-5 film (Kodak).For SDS–PAGE 1 µl of translated protein was loadedon a 12% SDS–acrylamide gel.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To determine whether SHP affects the activity of the 12 ${alpha}$ -hydroxylasepromoter, we transfected increasing amounts of an expressionplasmid containing the mouse SHP cDNA into HepG2 cells witha fixed amount of the 12 ${alpha}$ -hydroxylase promoter construct pGL3-R12 ${alpha}$ -865(16). Figure 1 shows that SHP strongly suppresses 12 ${alpha}$ -hydroxylasepromoter activity. The level of suppression was >5-fold when200 ng SHP expression plasmid was transfected, comparable tothe bile acid-mediated suppression observed in the same system(16).

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Figure 1. SHP represses the rat 12 ${alpha}$ -hydroxylase promoter–luciferase construct in HepG2 cells. HepG2 cells were co-transfected with the pGL3-R12 ${alpha}$ -865 construct and the indicated amounts of SHP expression plasmid. Data represent the means ± SD of three assays performed in duplicate.

The FTF sites within the 12 ${alpha}$ -hydroxylase promoter (16) overlapa DR-1 site that has recently been identified (17) as a functionalPPAR-binding site. Since DR-1 is the binding site for HNF-4,a receptor known to interact with SHP (11), we decided to investigatewhether HNF-4 could bind and activate the 12 ${alpha}$ -hydroxylase promoter.Moreover, we wanted to determine whether HNF-4 is involved inthe suppression of 12 ${alpha}$ -hydroxylase promoter activity by bileacids. Figure 2A shows that both FTF and HNF-4 bind to the 12 ${alpha}$ -hydroxylasepromoter, as demonstrated by supershift assays using HepG2 nuclearextracts and a specific HNF-4 antibody (lane 2). Anti-FTF antibodiesabolished FTF binding and produced no supershifted band (lane3), as expected, since the antibody was raised against a peptidecorresponding to the DNA-binding domain of FTF (16). To establishthe potential role of HNF-4 in 12 ${alpha}$ -hydroxylase promoter activity,we co-transfected the 12 ${alpha}$ -hydroxylase promoter construct pGL3-R12 ${alpha}$ -865together with an expression plasmid with the HNF-4 cDNA in thepresence and absence of the SHP expression plasmid. For recipientcells we used CV-1 cells, a non-liver cell line that has no12 ${alpha}$ -hydroxylase activity because of the lack of liver-specifictranscription factors. As a control, we used the FTF expressionplasmid that we have already shown can activate the 12 ${alpha}$ -hydroxylasepromoter (16). As seen in Figure 2B, HNF-4 is capable of activatingthe 12 ${alpha}$ -hydroxylase promoter almost as much as FTF (11- versus14-fold). Most importantly, overexpression of SHP eliminatedmost of the FTF activation, but did not reduce the HNF-4-mediatedactivation of 12 ${alpha}$ -hydroxylase promoter activity.

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Figure 2. SHP represses FTF-dependent, but not HNF-4-dependent, activation of the rat 12 ${alpha}$ -hydroxylase promoter. (A) A gel shift experiment was performed as described in Materials and Methods, using 1 µg HepG2 nuclear extract and the indicated antibodies. The 12 ${alpha}$ -hydroxylase promoter sequence with the FTF sites (boxed) and the DR-1 site (arrows) highlighted is shown at the bottom. An irrelevant IgG was used as control antibody (lane 4). (B) CV-1 cells were co-transfected with the pGL3-R12 ${alpha}$ -865 construct and the indicated amounts of FTF or HNF-4 and/or SHP expression plasmids. Data represent the means ± SD of three assays performed in duplicate.

To further test whether FTF is the factor required for bileacid-mediated regulation of 12 ${alpha}$ -hydroxylase expression, we usedHep3B cells, a hepatoma cell line in which the 12 ${alpha}$ -hydroxylasepromoter is poorly expressed. Consistent with the notion thatexpression of FTF is needed for both activity and bile acid-mediatedregulation of 12 ${alpha}$ -hydroxylase, CDCA did not regulate 12 ${alpha}$ -hydroxylasepromoter activity when transfected in the absence of other expressionplasmids (Table 1). However, overexpression of FTF increased12 ${alpha}$ -hydroxylase promoter activity 7.7-fold and provided sensitivityto CDCA, indicating that FTF is limiting in H3B cells. In contrast,HNF-4 overexpression also activated 12 ${alpha}$ -hydroxylase promoteractivity 2-fold, but showed no regulation by CDCA. To furtherprove that expression of intact FTF is required for bile acid-mediatedregulation, we overexpressed two FTF deletion plasmids. pCI-FTF ${Delta}$ LBDcontains a FTF cDNA with the ligand-binding domain deleted.The ligand-binding domain is known to be required for interactionof other nuclear receptors with different coactivators or corepressors.pCI-FTF ${Delta}$ LBD activated the 12 ${alpha}$ -hydroxylase promoter but did notsupport regulation by bile acids, suggesting that the FTF ligand-bindingdomain is involved in the interaction with SHP to provide regulation.pCI-FTF ${Delta}$ AF-2 is a FTF mutant with the C-terminal activation domaindeleted. Overexpression of this mutant decreased 12 ${alpha}$ -hydroxylaseactivity to undetectable levels, presumably by competing outendogenous FTF by the inert mutant.

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Table 1. Overexpression of FTF or FTF ${Delta}$ LBD increases 12 ${alpha}$ -hydroxylase promoter–luciferase construct activity in Hep3B cells

To further evaluate the specific roles of FTF and HNF-4 inboth 12 ${alpha}$ -hydroxylase promoter activity as well as for its bile acid-mediatedregulation, we attempted to create 12 ${alpha}$ -hydroxylase promoterslacking either a HNF-4 site or both FTF sites previously characterized(located between nucleotides –63 and –48) and transfectedthem into HepG2 cells that were incubated with and without CDCAto study both promoter activity and bile acid regulation (Fig.3A). FTF and HNF-4 binding to these mutants was tested by mobilityshift analysis using in vitro made proteins (Fig. 3B). Wild-type12 ${alpha}$ -hydroxylase binds both in vitro produced proteins, althoughwith very different affinities (Fig. 3B, lanes 2 and 3). HNF-4binds to the wild-type sequence, although with lower affinitythan HNF-4 from HepG2 cells (compare Fig. 3B, lane 3 with Fig.2A, lane 1). We then created two 12 ${alpha}$ -hydroxylase promoterconstructs with the HNF-4 site mutated. In one construct (Fig. 3A,12 ${alpha}$ -hydroxylase 5'-flanking DR-1 mutant) the three nucleotideslocated 5' of the two DR-1 repeats were mutated to maintainFTF but not HNF-4 binding, since these nucleotides are knownto be required for PPAR ${alpha}$ binding to the DR-1 site (17). Thismutant promoter had no detectable activity (Fig. 3A), presumablydue to lack of HNF-4 binding (Fig. 3B, lane 6). FTF binds tothis mutant essentially as to the wild-type (Fig. 3B, lanes5 and 2). The second mutant that we created, 12 ${alpha}$ -hydroxylaseFTF consensus, contained one FTF consensus site instead of two.We used the rat 7 ${alpha}$ -hydroxylase promoter FTF site (21) and the3' repeat was mutated (Fig. 3A) so that the 12 ${alpha}$ -hydroxylase HNF-4site was destroyed. This promoter mutant had no detectable activity(Fig. 3A) and, as expected, it is capable of binding FTF butnot HNF-4 (Fig. 3B, lanes 8 and 9). In an attempt to createa 12 ${alpha}$ -hydroxylase promoter mutant with a HNF-4 site but no FTFsites, we mutated the 12 ${alpha}$ -hydroxylase FTF/HNF-4 site to the apoproteinCIII C3P site (22,23) to create 12 ${alpha}$ -hydroxylase apoCIII C3P HNF-4(Fig. 3A). This promoter construct showed approximately one-thirdof the wild-type promoter activity and was slightly less regulatedby CDCA than the wild-type promoter (Fig. 3A). As expected,this mutant binds HNF-4 with greater affinity than the wild-type12 ${alpha}$ -hydroxylase site (Fig. 3B, lane 12). Unexpectedly, this mutantstill binds FTF (Fig. 3B, lane 11). Close examination of thesequence revealed that it contains a reversed FTF site with8 of 9 nt conserved (Fig. 3A). Multiple attempts to create amutant that would bind HNF-4 but not FTF based either on the12 ${alpha}$ -hydroxylase FTF/HNF-4 site or the apoprotein CIII C3P sitewere unsuccessful.

To additionally evaluate the effect of SHP on regulation ofthe 12 ${alpha}$ -hydroxylase promoter, we overexpressed wild-type SHPand a deletion mutant that lacks the C-terminus of the SHP protein,SHP ${Delta}$ 160X(1–159) (11), in CV-1 cells. The C-terminus ofSHP contains a domain that is required for repression of nuclearreceptors, such as HNF-4. Figure 4 shows that SHP suppressedFTF-dependent activation of the 12 ${alpha}$ -hydroxylase promoter in adose-dependent manner. However, when the SHP deletion mutantwas used, no suppression was observed.

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Figure 4. SHP repression of FTF-dependent activation of the rat 12 ${alpha}$ -hydroxylase promoter in CV-1 cells requires the SHP repression domain. CV-1 cells were co-transfected with the 12 ${alpha}$ -hydroxylase promoter construct and the indicated amounts of FTF and either wild-type SHP or SHPW160(1–159) (11), a SHP cDNA with the suppression domain deleted, as indicated in the figure. Data represent the means ± SD of three assays performed in duplicate.

It has been previously shown that FTF and SHP interact in vivo(7,8) but the domains required for that interaction are unknown.To characterize the potential distinctive domain(s) requiredfor this interaction, we performed two-hybrid assays in mammaliancells. We co-expressed a VP16–FTF fusion construct andseveral GAL4–SHP fusion constructs, as shown in Figure5. When a GAL4 fusion construct was used that contained thefull-length SHP cDNA, an interaction was observed as indicatedby an 8-fold activation when compared with the empty pVP16 vector.However, deletion of any SHP domain eliminated that activation.As a control we used the same GAL4–SHP constructs witha pVP16-HNF-4 plasmid. GAL4–SHP constructs that containedthe putative interaction domain were capable of interactionwith HNF-4 as described (11), suggesting that the modes of interactionof SHP with HNF-4 and FTF are different.

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Figure 5. FTF requires an intact SHP protein for the interaction between them in vivo. pVP16-FTF and previously described pGAL4-SHP mutants (12) were used in a mammalian two-hybrid assay in CV-1 cells. Five hundred nanograms of each pVP16-FTF, or pVP16 as a control, and each pGAL4-SHP construct were transfected together with 100 ng thymidine kinase promoter–luciferase reporter plasmid containing four GAL4-binding sites and pCMV-gal as a control for transfection efficiency. As a positive control, pVP16-HNF-4 was used with each pGAL4-SHP plasmid. The x-axis shows the different GAL4–SHP mutants used and the numbers correspond to the SHP amino acid number included in each construct. The y-axis represents the fold activation compared with the activity of an empty pVP16 vector. The scheme at the bottom represents the GAL4–SHP fusion protein showing the different SHP domains and the amino acid numbers that expand each domain. Data represent the means ± SD of three assays performed in duplicate.

To gain further insight into the mechanism of action of SHPrepression on the 12 ${alpha}$ -hydroxylase promoter, we performed gelshift experiments using in vitro produced FTF in the absenceor presence of SHP. Figure 6 shows that SHP prevents bindingof FTF to the 12 ${alpha}$ -hydroxylase promoter in a linear fashion tothe point that FTF binding is essentially eliminated (lanes2–5). We included [³⁵S]methionine in the synthesis reactions,in order to quantify actual protein synthesis and to ensurethat the diminished binding was not due to less FTF synthesized.Although FTF synthesis was slightly diminished when the SHPplasmid was included in the in vitro synthesis reaction (lanes7–10), FTF binding decreased to a much greater degree.

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Figure 6. FTF binding to the 12 ${alpha}$ -hydroxylase promoter is prevented by SHP. Gel shift experiments (lanes 1–5) using the 12 ${alpha}$ -hydroxylase promoter probe and SDS–acrylamide gels (lanes 6–10) were performed as described in Materials and Methods, using in vitro synthesized FTF and SHP proteins or in vitro produced GHR as a control. The number of micrograms refers to the amount of the corresponding plasmid used in the protein synthesis reaction. The GHR plasmid was also used to bring the amount of T7 promoter-containing plasmids to a total of 1 µg. The wild-type FTF/HNF-4 site from the 12 ${alpha}$ -hydroxylase promoter was used as probe for the gel shift with FTF alone (lane 2) or with different amounts of SHP (lanes 3–5). Protein samples used for the gel retardation were analyzed in a SDS gel (lanes 6–10).

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In this study we present evidence that SHP inhibits 12 ${alpha}$ -hydroxylaseexpression through the FTF orphan receptor and not through HNF-4,in spite of HNF-4 being an activator of 12 ${alpha}$ -hydroxylase transcriptionthat is required for 12 ${alpha}$ -hydroxylase promoter activity and ofHNF-4 being capable of interacting with SHP. We also providedata that show that SHP prevents binding of FTF to the12 ${alpha}$ -hydroxylase promoter site. Finally, we have determined theFTF and SHP domains that are responsible for interaction betweenthese two proteins.

Recent studies have implicated SHP as the factor responsiblefor bile acid-mediated suppression of 7 ${alpha}$ -hydroxylase transcription(7,8), the rate-limiting enzyme in the classic pathway for bileacid synthesis. These studies used mammalian two-hybrid systemsand GST pull-down assays to demonstrate that FTF and SHP interactboth in vivo and in vitro. They also showed that overexpressionof SHP can override FTF-mediated transactivation of 7 ${alpha}$ -hydroxylasepromoter activity when both FTF and SHP expression plasmidswere co-transfected with a 7 ${alpha}$ -hydroxylase promoter constructin a non-liver cell line (7,8). In the present studies we haveshown that SHP overturns FTF-mediated activation of 12 ${alpha}$ -hydroxylasewhen co-transfected in a non-liver cell line (Figs 2 and 4).SHP is also capable of suppressing the 12 ${alpha}$ -hydroxylase promoterin HepG2 cells without the need for overexpression of co-transfectedFTF cDNA (Fig. 1).

SHP is a repressor of several nuclear receptors, such as RXR(10), ER (12) and HNF-4 (11). Of particular interest is theinteraction between HNF-4 and SHP, because HNF-4 has been shownto activate the 7 ${alpha}$ -hydroxylase promoter (18) through bindingto a DR-1 element that overlaps the FTF site (6,21). Interestingly,the 12 ${alpha}$ -hydroxylase promoter also has a DR-1 element overlappingthe FTF sites recently localized in our laboratory (16), andthis site binds PPAR ${alpha}$ , another nuclear receptor (17). These observationsraised the question as to whether HNF-4 could be the major transcriptionfactor that interacts with SHP and mediates transcriptionalregulation of the 7 ${alpha}$ -hydroxylase and 12 ${alpha}$ -hydroxylase genes bybile acids. To date, HNF-4 has not been eliminated as a majortranscription factor mediating repression of 7 ${alpha}$ -hydroxylase and12 ${alpha}$ -hydroxylase by bile acids. Indeed, we show that HNF-4 bindsto the 12 ${alpha}$ -hydroxylase promoter, as demonstrated by supershiftassays (Figs 2A and 3B). HNF-4 also activates the 12 ${alpha}$ -hydroxylasepromoter in a non-liver cell line (Fig. 2B, lane 4), but overexpressionof SHP cannot override this activation (Fig. 2A, lane 5). Additionally,the experiments shown in Figure 3 demonstrate the key rolesof both HNF-4 and FTF in the activity of the 12 ${alpha}$ -hydroxylasepromoter. Indeed, 12 ${alpha}$ -hydroxylase promoter mutants that lackHNF-4 binding had no detectable activity.

FTF binding is also important for 12 ${alpha}$ -hydroxylase promoter activity,although not as much as HNF-4. A 12 ${alpha}$ -hydroxylase mutant thatbinds HNF-4 with much higher activity than the wild-type promoterand binds FTF with about half the affinity of the wild-type(12 ${alpha}$ -hydroxylase apoCIII C3P HNF-4) had about one-third of thewild-type promoter activity (Fig. 3A). This promoter mutantis regulated by bile acids slightly less than the wild-typepromoter, probably because of less FTF binding (Fig. 3B, lane11). If HNF-4 were implicated in bile acid-mediated regulationof the 12 ${alpha}$ -hydroxylase promoter, the 12 ${alpha}$ -hydroxylase apoCIII C3PHNF-4 mutant would be expected to be more regulated by bileacids than the wild-type promoter, not less. Unfortunately wehave not been able to create a mutant that would bind HNF-4but not FTF, probably because of homology between the FTF andHNF-4 binding sites. Such a mutant would be useful to furtherrule out any involvement of HNF-4 in the regulation of 12 ${alpha}$ -hydroxylasepromoter activity by bile acids and support the overexpressionexperiments shown in Figure 2B and Table 1. As we demonstratedearlier, FTF also activates the 12 ${alpha}$ -hydroxylase promoter in CV-1cells (16) but, in contrast to HNF-4 activation, this FTF-mediatedactivation can be overridden by overexpression of SHP (Fig.2B, lanes 2 and 3). Together these results show that FTF isthe nuclear receptor that interacts with SHP to provide suppressionof 12 ${alpha}$ -hydroxylase. How both FTF and HNF-4 can bind to theiroverlapping sites so that 12 ${alpha}$ -hydroxylase expression is sustainedby HNF-4 and regulated by the interaction between FTF and SHPremains to be studied. It is important to point out that thepromoter of the 7 ${alpha}$ -hydroxylase gene, a gene whose expressionis coordinately regulated with 12 ${alpha}$ -hydroxylase by bile acids(15), also contains an overlapping FTF site and DR-1 element(21).

We used Hep3B cells to further demonstrate that FTF is thefactor that interacts with SHP to mediate regulation of 12 ${alpha}$ -hydroxylasetranscription by bile acids (Table 1). Hep3B cells have low12 ${alpha}$ -hydroxylase promoter activity that does not respond to CDCA(Table 1), most likely because FTF and HNF-4 are expressed atlow levels (24). This is analogous to the lack of bile acid-mediatedregulation of 7 ${alpha}$ -hydroxylase expression in the absence of a FXRexpression plasmid in HepG-2 cells (25) and in primary hepatocyeswhen they are transfected with relatively high amounts of 7 ${alpha}$ -hydroxylasepromoter plasmid (21). In those cases the lack of regulationwas overcome by transfecting a FXR expression plasmid. In Hep3Bcells overexpression of FTF not only activated the 12 ${alpha}$ -hydroxylasepromoter but also provided regulation by bile acids (Table 1).Regulation of the 12 ${alpha}$ -hydroxylase promoter by bile acids is lowerin Hep3B cells than that seen in HepG2 cells (16), probablydue to a relatively low expression of SHP in Hep3B cells ascompared with HepG2 cells. Overexpression of SHP provides furthersuppression of 12 ${alpha}$ -hydroxylase in Hep3B cells (data not shown),although this was further studied in CV-1 cells (Fig. 4). Onthe other hand, HNF-4 activation of the 12 ${alpha}$ -hydroxylase promoterwas not regulated by bile acids, supporting the notion thatFTF is the factor that interacts with SHP to mediate regulationby bile acids.

Overexpressing two FTF mutants provided preliminary characterizationof the FTF domains involved in the activation or bile acid-mediatedregulation of 12 ${alpha}$ -hydroxylase. FTF ${Delta}$ AF-2, a mutant that has theactivation domain AF-2 deleted, did not activate the 12 ${alpha}$ -hydroxylasepromoter. In fact, this mutant eliminated even the low basalactivity, acting as a dominant negative mutant similar to observationswith the hepatitis virus core promoter (24). Another FTF mutantwith its ligand-binding domain deleted (FTF ${Delta}$ LBD) mediated transactivationof the 12 ${alpha}$ -hydroxylase promoter. However, bile acids could notregulate its activity, suggesting that the FTF ligand-bindingdomain acts as an interacting domain with SHP (Table 1).

An important issue that has yet to be explored is the molecularmechanism involved in the suppression of FTF transactivationby SHP. Different mechanisms have been elucidated for the interactionof SHP with other nuclear receptors. It has been shown thatSHP contains a repressor domain in its C-terminal region thatcould function on RXR, ER and HNF-4 (11–13). Our resultssupport the functionality of the SHP repressor domain on transactivationof the 12 ${alpha}$ -hydroxylase promoter by FTF since a SHP mutant withno suppressor domain did not prevent FTF-mediated activationof the 12 ${alpha}$ -hydroxylase promoter in CV-1 cells (Fig. 4). However,the mechanism of action for SHP suppression appears to be differenton FTF transactivation than on other nuclear receptors. First,there is no distinctive domain in SHP sufficient for interactionwith FTF. Two-hybrid experiments in mammalian cells show thata fully intact SHP protein is required for its interaction withFTF (Fig. 5). In contrast, only amino acids 92–148 inthe SHP protein are required for the interaction with RXR orHNF-4 (11,12). This discrepancy was confirmed by carrying outcontrol experiments in parallel with the same SHP mutants andHNF-4. These results corroborate a different interaction betweenSHP and FTF, and SHP and HNF-4 (Fig. 5).

Our studies add FTF, to the list of nuclear receptors whosebinding to its DNA target is prevented by SHP. Interaction betweenSHP and FTF prevents binding of FTF to its binding site withinthe 12 ${alpha}$ -hydroxylase promoter (Fig. 6). This observation is similarto the effect of SHP on binding of the RAR–RXR heterodimerto its recognition site (10), but different to the lack of effectof SHP on binding of ER to its DNA element (13). It needs tobe investigated whether inhibition of FTF binding by SHP isa general mechanism for bile acid-regulated genes, such as 7 ${alpha}$ -hydroxylase,and whether this prevention of binding of FTF to its targetDNA is the only mechanism of action for the repression of FTFtransactivation by SHP. In other receptors, such as HNF-4, SHPrepresses receptor-mediated transactivation via two separatesteps, i.e. competition with coactivators and a directeffect of its transcriptional repressor function. It is possiblethat SHP represses FTF transactivation by more than one mechanism.

In summary, these studies show the key roles of HNF-4 and FTFin expression of the 12 ${alpha}$ -hydroxylase gene. They also add furthersupport to FTF being the SHP target involved in bile acid-mediatedregulation of gene transcription and rule out HNF-4 as sucha target, at least for the 12 ${alpha}$ -hydroxylase gene. In addition,our studies provide important insights into the mechanisms ofaction of FTF and SHP on the regulation of gene transcriptionby bile acids.

ACKNOWLEDGEMENTS

Stacy Beck provided invaluable technical help. We thank Dr LucBélanger for suggestions and for plasmids pCI-FTF, pCI-FTF ${Delta}$ LBDand pCI-FTF ${Delta}$ AF-2, Drs David Moore and Yoon-Kwang Lee for SHPplasmids and Dr David W. Russell for anti-FTF antibodies. Weare grateful to Dr Hylemon for critical comments and support.We also thank Dr Wells for discussions and critical review ofthe manuscript. This research was supported in part by AmericanHeart Association Grant-in-Aid 9950042N and National Institutesof Health Grants DK44218 and DK 38030.

FOOTNOTES

^* To whom correspondence should be addressed. Tel: +1 804 8280140; Fax: +1 804 828 0676; Email: ggil{at}vcu.edu

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell

[ISI]

[Medline]

2 Javitt,N.B. (1994) Bile acid synthesis from cholesterol: regulatory and auxiliary pathways. FASEB J., 8, 1308–1311.[Abstract]

3 Eggertsen,G., Olin,M., Andersson,U., Ishida,H., Kubota,S., Hellman,U., Okuda,K.-I. and Björkhem,I. (1996) Molecular cloning and expression of rabbit sterol 12 ${alpha}$ -hydroxylase. J. Biol. Chem., 271, 32269–32275.[Abstract/Free Full Text]

4 Nuclear Receptors Nomenclature Committee (1999) A unified nomenclature system for the nuclear receptor superfamily. Cell, 97, 161–163.[ISI][Medline]

5 Galarneau,L., Pare,J.F., Allard,D., Hamel,D., Levesque,L., Tugwood,J.D., Green,S. and Belanger,L. (1996) The alpha1-fetoprotein locus is activated by a nuclear receptor of the Drosophila FTZ-F1 family. Mol. Cell. Biol., 16, 3853–3865.[Abstract]

6 Nitta,M., Ku,S., Brown,C., Okamoto,A.Y. and Shan,B. (1999) CPF: an orphan nuclear receptor that regulates liver-specific expression of the human cholesterol 7 ${alpha}$ -hydroxylase gene. Proc. Natl Acad. Sci. USA, 96, 6660–6665.[Abstract/Free Full Text]

7 Goodwin,B., Jones,S.A., Price,R.R., Watson,M.A., McKee,D.D., Moore,L.B., Galardi,C., Wilson,J.G., Lewis,M.C., Roth,M.E. et al. (2000) A regulatory cascade of the nuclear receptors FXR, SHP-1 and LRH-1 represses bile acid biosynthesis. Mol. Cell, 6, 517–526.[ISI][Medline]

8 Lu,T.T., Makishima,M., Repa,J.J., Schoonjans,K., Kerr,T.A., Auwerx,J. and Mangelsdorf,D.J. (2000) Molecular basis for feedback regulation of bile acid synthesis by nuclear receptors. Mol. Cell, 6, 507–515.[ISI][Medline]

9 Gupta,S., Stravitz,R.T., Dent,P. and Hylemon,P.B. (2001) Down-regulation of cholesterol 7 ${alpha}$ -hydroxylase (CYPA1) gene expression by bile acids in primary rat hepatocytes is mediated by the c-Jun N-terminal kinase pathway. J. Biol. Chem., 276, 15816–15822.[Abstract/Free Full Text]

10 Seol,W., Choi,H.S. and Moore,D.D. (1996) An orphan nuclear hormone receptor that lacks a DNA binding domain and heterodimerizes with other receptors. Science, 272, 1336–1339.[Abstract]

11 Lee,Y.K., Dell,H., Dowhan,D.H., Hadzopoulou-Cladaras,M. and Moore,D.D. (2000) The orphan nuclear receptor SHP inhibits hepatocyte nuclear factor 4 and retinoid X receptor transactivation: two mechanisms for repression. Mol. Cell. Biol., 20, 187–195.[Abstract/Free Full Text]

12 Seol,W., Chung,M. and Moore,D.D. (1997) Novel receptor interaction and repression domains in the orphan receptor SHP. Mol. Cell. Biol., 17, 7126–7131.[Abstract]

13 Seol,W., Hanstein,B., Brown,M. and Moore,D.D. (1998) Inhibition of estrogen receptor action by the orphan receptor SHP (short heterodimer partner). Mol. Endocrinol., 12, 1551–1557.[Abstract/Free Full Text]

14 Andersson,U., Yang,Y.Z., Bjorkhem,I., Einarsson,C., Eggertsen,G. and Gafvels,M. (1999) Thyroid hormone suppresses hepatic sterol 12alpha-hydroxylase (CYP8B1) activity and messenger ribonucleic acid in rat liver: failure to define known thyroid hormone response elements in the gene. Biochim. Biophys. Acta, 1438, 167–174.[Medline]

15 Vlahcevic,Z.R., Eggerten,G., Björkhem,I., Hylemon,P.B., Redford,K. and Pandak,W.M. (2000) Regulation of sterol 12 ${alpha}$ -hydroxylase and cholic acid biosynthesis in the rat. Gastroenterology, 118, 599–607.[ISI][Medline]

16 del Castillo-Olivares,A. and Gil,G. (2000) ${alpha}$ ₁-Fetoprotein transcription factor is required for the expression of sterol 12 ${alpha}$ -hydroxylase, the specific enzyme for cholic acid synthesis. J. Biol. Chem., 275, 17793–17799.[Abstract/Free Full Text]

17 Hunt,M.C., Yang,Y.Z., Eggertsen,G., Carneheim,C.M., Gafvels,M., Einarsson,C. and Alexson,S.E. (2000) The peroxisome proliferator-activated receptor alpha (PPARalpha) regulates bile acid biosynthesis. J. Biol. Chem., 275, 28947–28953.[Abstract/Free Full Text]

18 Stroup,D. and Chiang,J.Y. (2000) HNF4 and COUP-TFII interact to modulate transcription of the cholesterol 7alpha-hydroxylase gene (CYP7A1). J. Lipid Res., 41, 1–11.[Abstract/Free Full Text]

19 Subramanian,A., Teixeira,J., Wang,J. and Gil,G. (1995) A STAT factor mediates the sexually dimorphic regulation of hepatic cytochrome P450 3A10/lithocholic acid 6ß-hydroxylase gene expression by growth hormone. Mol. Cell. Biol., 15, 4672–4682.[Abstract]

20 Subramanian,A., Wang,J. and Gil,G. (1998) STAT-5 and NF-Y are involved in expression and growth hormone-mediated sexually dimorphic regulation of cytochrome P450 3A10/lithocholic acid 6ß-hydroxylase. Nucleic Acids Res., 29, 2173–2178.

21 del Castillo-Olivares,A. and Gil,G. (2000) Role of FXR and FTF on the bile acid-mediated suppression of cholesterol 7 ${alpha}$ -hydroxylase transcription. Nucleic Acids Res., 28, 3587–3593.[Abstract/Free Full Text]

22 Leff,T., Reue,K., Melian,A., Culver,H. and Breslow,J.L. (1989) A regulatory element in the ApoCIII promoter that directs hepatic specific transcription binds to proteins in expressing and nonexpressing cell types. J. Biol. Chem., 264, 16132–16137.[Abstract/Free Full Text]

23 Ladias,J.A., Hadzopoulou-Cladaras,M., Kardassis,D., Cardot,P., Cheng,J., Zannis,V. and Cladaras,C. (1992) Transcriptional regulation of human apolipoprotein genes ApoB, ApoCIII and ApoAII by members of the steroid hormone receptor superfamily HNF-4, ARP-1, EAR-2 and EAR-3. J. Biol. Chem., 267, 15849–15860.[Abstract/Free Full Text]

24 Gilbert,S., Galarneau,L., Lamontagne,A., Roy,S. and Belanger,L. (2000) The hepatitis B virus core promoter is strongly activated by the liver nuclear receptor fetoprotein transcription factor or by ectopically expressed steroidogenic factor 1. J. Virol., 74, 5032–5039.[Abstract/Free Full Text]

25 Makishima,M., Okamoto,A.Y., Repa,J.J., Tu,H., Learned,R.M., Luk,A., Hull,M.V., Lustig,K.D., Mangelsdorf,D.J. and Shan,B. (1999) Identification of a nuclear receptor for bile acids. Science, 284, 1362–1365.[Abstract/Free Full Text]

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				J. Zhang, W. Huang, M. Qatanani, R. M. Evans, and D. D. Moore The Constitutive Androstane Receptor and Pregnane X Receptor Function Coordinately to Prevent Bile Acid-induced Hepatotoxicity J. Biol. Chem., November 19, 2004; 279(47): 49517 - 49522. [Abstract] [Full Text] [PDF]

				T. Nishimaki-Mogami, M. Une, T. Fujino, Y. Sato, N. Tamehiro, Y. Kawahara, K. Shudo, and K. Inoue Identification of intermediates in the bile acid synthetic pathway as ligands for the farnesoid X receptor J. Lipid Res., August 1, 2004; 45(8): 1538 - 1545. [Abstract] [Full Text] [PDF]

				D. Jung, B. Hagenbuch, M. Fried, P. J. Meier, and G. A. Kullak-Ublick Role of liver-enriched transcription factors and nuclear receptors in regulating the human, mouse, and rat NTCP gene Am J Physiol Gastrointest Liver Physiol, May 1, 2004; 286(5): G752 - G761. [Abstract] [Full Text] [PDF]

Nucleic Acids Research

Suppression of sterol 12-hydroxylase transcription by the short heterodimer partner: insights into the repression mechanism

Suppression of sterol 12 ${alpha}$ -hydroxylase transcription by the short heterodimer partner: insights into the repression mechanism