Activation of the Mouse TATA-less and Human TATA-Containing UDP-Glucuronosyltransferase 1A1 Promoters by Hepatocyte Nuclear Factor 1

QUICK SEARCH:

[advanced]

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

This Article

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

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Bernard, P.
	Articles by Wahli, W.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Bernard, P.
	Articles by Wahli, W.

Vol. 56, Issue 3, 526-536, September 1999

Activation of the Mouse TATA-less and Human TATA-Containing UDP-Glucuronosyltransferase 1A1 Promoters by Hepatocyte Nuclear Factor 1¹

Pascal Bernard, Hervé Goudonnet, Yves Artur, Béatrice Desvergne, and Walter Wahli

Institut de Biologie Animale, Bâtiment de Biologie, Université de Lausanne, Lausanne, Switzerland (P.B., B.D., W.W.); and Laboratoire de Biochimie Pharmacologique, Unité de Formation et de Recherche Pharmacie, Université de Bourgogne, Dijon, France (P.B., H.G., Y.A.)

	Summary

Top Summary Introduction Experimental Procedures Results Discussion References

UDP-glucuronosyltransferase (UGT) 1A1 (UGT1A1) catalyzes the glucuronidation of bilirubin in liver. Among all UGT isoformsidentified to date, it is the only relevant bilirubin-glucuronidatingenzyme in human. Because glucuronoconjugation is the major routeof bilirubin elimination, any genetic alteration that affectsbilirubin glucuronosyltransferase activity may result in a moreor less severe hyperbilirubinemia. In this study, we report thecloning and characterization of the transcriptional regulationof the mouse UGT1A1 gene. Primary-structure analysis of the mouseThymidine Adevice promoter revealed marked differences with itshuman homolog. First, the mouse promoter lacks the highly polymorphicthymidine/adenine repeat occurring in the human promoter, whichhas been associated with some forms of hyperbilirubinemia. Second,an L1 transposon element, which is absent in the human promoter,is found 480 bp upstream of the transcription start site in mouse.Using the electromobility shift and DNase I footprinting experiments,we have identified a hepatocyte nuclear factor 1-binding sitein the mouse UGT1A1 promoter that confers responsiveness to bothfactors HNF1 $alpha$ and HNF1 $beta$ in HEK293 cells. Furthermore, we showthat this element, which is conserved in the human promoter, alsoconfers strong HNF1 responsiveness to the human UGT1A1 gene. Together,these results provide evidence for a major regulatory functionof this liver-enriched transcription factor in UGT1A1 activityin both rodents andhuman.

	Introduction

Top Summary Introduction Experimental Procedures Results Discussion References

In mammals, detoxification of the hydrophobic bilirubin occurs mainly in the liver via its conjugation with uridine diphosphateglucuronic acid. This reaction, which is catalyzed by microsomalUDP-glucuronosyltransferases (UGTs) (EC 2.4.1.17) produces hydrophilicbilirubin-mono- and diconjugates that are excreted at high ratesin the bile (Hauser and Gollan, 1990; Jansen et al., 1992). UGTsare produced by a multigene superfamily with specificity for avariety of endogenous substrates and xenobiotics. Mammalian UGTsare subdivided into two groups, the UGT1 and the UGT2 families.UGT1 family members are encoded by a particularly complex geneof about 500 kb ("the UGT1 cluster," Mackenzie et al., 1997).It consists of multiple related homologous unique first exons(exon 1), which encode the isoform specific N terminus of theenzymes. The C-terminal part is encoded in a single set of fourexons (exons 2-5), which is common to all UGT1 isoforms (Ritteret al., 1992; Emi et al., 1995; Mackenzie et al., 1997). A promoterregion with its regulatory elements is thought to be located upstreamof each unique first exon, but, for several of them, this regionhas not yet been characterized (Ritter et al., 1992).

The UGT1A1 isoform is likely to be the major isoform involved in bilirubin detoxification in human (Bosma et al., 1994). Inheriteddisorders that decrease or suppress UGT1A1 expression result inunconjugated bilirubin accumulation. Mild forms of unconjugatedhyperbilirubinemia are known as Gilbert and Crigler-Najjar typeII syndromes, whereas in more severe forms, the Crigler-Najjartype I disease can be fatal (Aono et al., 1995; Bosma et al.,1995). Some of the mutations causing these disorders are localizedin the common exons 2 to 5, leading to an alteration of all isoformsproduced by the UGT1 locus (reviewed in Mackenzie et al., 1997).Others are in exon 1A1 and thus alter only UGT1A1 activity. Thusfar, the UGT1A1*28 polymorphism is the only genetic variationreported in a regulatory region of the gene. It is responsiblefor most Gilbert's disease cases (Bosma et al., 1995). This polymorphismconcerns the six-thymidine/adenine (TA) track in the wild-typeUGT1A1 promoter, which is replaced by five, seven, or eight TArepeats in the altered genes, whose activity is inversely correlatedwith the length of the track (Beutler et al., 1998). Expressionof the human UGT1A1 mRNA is primarily in the liver but can alsobe detected in biliary and colon epithelia (Ritter et al., 1992;Strassburg et al., 1997, 1998). In rat, the tissue distributionis similar in liver and intestine. In addition, UGT1A1 is alsoexpressed at low levels in kidney, which is not the case in human(Ritter et al., 1992; Emi et al., 1995).

Surprisingly, only the promoter of the human UGT1A1 gene has been sequenced thus far. However, with the exception of the TAtrack, no functional promoter characterization has been performed(Brierley et al., 1996). The broad use of mice and rats as laboratoryanimals for pharmacological studies has prompted us to investigateUGT1A1 transcriptional regulation in the mouse, not least becausethe gene knockout technology is now well mastered for this animaland might be applied later to the UGT1 locus once characterized.Moreover, studies using this technology provided evidence fora role of liver-enriched transcription factors in UGT1A1 expression.The inactivation of the HNF1 $alpha$ gene resulted in a mild hyperbilirubinemia,which, according to the above-mentioned observations, might reflectan altered UGT1A1 gene expression (Pontoglio et al., 1996). Similarly,knock-out of C/EBP $alpha$ in mouse liver affects UGT1A1 gene expressionresulting in a severe toxic hyperbilirubinemia (Lee et al., 1997).These observations, together with UGT1A1 being the main isoformfrom the UGT1 locus expressed in rat liver (Emi et al., 1995),argue strongly for a crucial role of the UGT1A1 isoform in bilirubindetoxification in rodents. Recently, other studies have highlightedthe important role of HNF1 $alpha$ and C/EBP $alpha$ in regulating the transcriptionof the rat UGT2B1 isoform (Hansen et al., 1997, 1998). In contrast,nothing is presently known of the mechanisms of transcriptionalregulation of the UGT1A1 gene by these factors, although theirinvolvement has been suggested, as mentionedabove.

To better understand the physiological role of the UGT1A1 isoform in the mouse, we have isolated the UGT1A1 gene. Its promoterwas then compared with that of the human gene, which revealedthe lack of a TATA box in the mouse promoter. Furthermore, evidenceis provided for a direct involvement of HNF1 in the regulationof the mouse and human UGT1A1promoters.

	Experimental Procedures

Top Summary Introduction Experimental Procedures Results Discussion References

Materials. The expression plasmids pRSV-HNF1 $alpha$ and pRSV-HNF1 $beta$ were a kind gift from Dr. Moshe Yaniv (Unité des Virus Oncogènes, InstitutPasteur, Paris, France). The $alpha$ -HCt-284 polyclonal antiserum directedagainst HNF1 $alpha$ (Chouard et al., 1997) was a kind gift from Dr.Marco Pontoglio (Unité des Virus Oncogènes, Institut Pasteur,Paris, France) and Dr. Moshe Yaniv. All UGT1A1 nucleotide sequencesused were numbered relative to the major transcription start sitedetermined in thisstudy.

Isolation and Characterization of Genomic and cDNA Clones. A portion (1 × 10⁶ plaque-forming units) of a mouse L129/SVJ genomic DNA library in $lambda$ FIXII (Clontech Laboratories, Palo Alto,CA) were screened with two oligonucleotides complementary to themouse UGT1A1 cDNA (Chu et al., 1997) as probes. Two clones ( $lambda$ mPGT1A1-1, $lambda$ mPGT1A1-2) were isolated, plaque-purified, and characterizedby polymerase chain reaction (PCR) and restriction enzyme analysis.From the $lambda$ mPGT1A1-1 clone, a 2.4-kb XbaI restriction fragmentcontaining the UGT1A1 first exon was subcloned in the pBluescriptKSII vector, yielding the pKS-1A1 genomic subclone. DNA was sequencedon both strands by the dideoxy termination method using T7 DNApolymerase (T7 sequencing kit; Pharmacia Biotech Europe, Dübendorf,Switzerland). The cDNA clones were obtained by screening 1 × 10⁶ plaque-forming units of an adult mouse liver 5'-extended cDNAlibrary in $lambda$ gt10 with the same oligonucleotides as indicated above,yielding 10 independent clones. Similarly, a 15-day-old embryonicmouse 5'-extended cDNA library in $lambda$ gt10 was screened followingthe same procedure, yielding one clone. After PCR amplificationusing phage-specific oligonucleotides, the 11 independent cloneswere subcloned into the pBluescript vector for subsequent sequencing.The human UGT1A1 promoter was cloned by PCR on human genomic DNAand subcloned into the pBLCAT3 vector yielding the $-$ 617/+15 hUGT1A1-chloramphenicolacetyltransferase (CAT) construct. The construct was sequencedon both strands. Its sequence is identical with that publishedpreviously (Brierley et al., 1996) except for the length of theTA repeat in the polymorphic TATA box, which is (TA)₅TAA insteadof (TA)₆TAA (Beutler et al., 1998).

RNA Isolation and Primer Extension Analysis. Total RNA was isolated from mouse liver by the phenol and guanidine isothiocyanate method following the supplier's instructions(Trizol reagent; Life Technologies, Basel, Switzerland). An end-labeledantisense oligonucleotide primer complementary to nucleotides+95/+120 of the UGT1A1 gene was hybridized to 50 µg of total RNAfor 1 h at 42°C in 50 mM Tris-HCl (pH 8.3), 8 mM MgCl₂, 30 mMKCl, 10 mM DTT in a final volume of 50 µl. The primer-annealedRNA was then subjected to extension by adding 2 mM each dNTP and25 units of avian myeloblastosis virus-reverse transcriptase (PharmaciaBiotech Europe, Dübendorf, Switzerland) for 1 h at 42, 44, or46°C. The reaction was stopped by addition of 50 mM EDTA and 15µg of Rnase Avian myeloblastosis virus (Boehringer Manheim, Rotkreuz,Switzerland) and incubated for 1 h at 37°C. The reaction productswere resolved on a 7 M urea, 8% polyacrylamide-1× Tris-borate-EDTAsequencinggel.

RNase Protection. A DNA fragment corresponding to nucleotide $-$ 76/+336 of the UGT1A1 gene was generated by PCR (Expand High Fidelity PCR system;Boehringer Mannheim, Rotkreuz, Switzerland) using the pKS-1A1genomic subclone as a template and cloned into the pBluescriptvector to obtain the pKS-RPA-1A1 construct. A 293-bp radiolabeledantisense riboprobe was generated from this plasmid. The riboprobe(0.5 × 10⁵ cpm) was mixed with 20 µg of total mouse liver RNA in 30 µl containing40 mM PIPES (pH 6.4), 1 mM EDTA, 400 mM NaCl, and 80% formamide.After overnight hybridization at 42°C, the samples were digestedwith 300 µl of RNase mix containing 300 mM NaCl, 10 mM Tris-HCl(pH 7.4), 5 mM EDTA, 2 µg/ml RNase T1 (Life Technologies, Inc.,Basel, Switzerland), and 40 µg/ml RNase A (Boehringer Mannheim)for 30 min at 30°C. The reaction was stopped by addition of 100µg of proteinase K (Boehringer Mannheim). The samples were resolvedon a 7 M urea, 8% polyacrylamide-1× Tris-borate-EDTA sequencinggel.

Generation of UGT1A1 Promoter Deletion Constructs and Site-Directed Mutagenesis. Four reporter genes encompassing different lengths of the UGT1A1 promoter were generated by PCR using the pKS-1A1 genomicsubclone as a template. The 5'-sense oligonucleotide primers usedwere complementary to the nucleotides $-$ 455 to $-$ 436, $-$ 93 to $-$ 74,and $-$ 44 to $-$ 25 of the cloned genomic sequence. The longest construct(from $-$ 1,074) was obtained using a vector-specific oligonucleotideprimer. The common 3'-antisense oligonucleotide used was complementaryto nucleotides $-$ 2 to +19 of the cloned genomic sequence. The PCRproducts were subcloned into the promoterless vector pBLCAT3,yielding the following plasmids: $-$ 1074/+19-mUGT1A1-CAT; $-$ 455/+19-mUGT1A1-CAT; $-$ 93/+19-mUGT1A1-CAT; and $-$ 44/+19-mUGT1A1-CAT. Point mutationswere introduced into the $-$ 455/+19 mUGT1A1-CAT plasmid (designatedWT-mUGT1A1-CAT in Fig. 8), at specific regulatory elements byPCR using the QuikChange site-directed mutagenesis kit (Stratagene,Basel, Switzerland) following the manufacturer's instructions.The three mutant plasmids were designated $Delta$ HNF1-mUGT1A1-CAT, $Delta$ Sp1-mUGT1A1-CAT,and $Delta$ Sp1/HNF1-mUGT1A1-CAT; the integrity of each was validatedby sequencing. The same procedure was used to mutate the HNF1site of the $-$ 617/+15-hUGT1A1-CAT plasmid (designated WT-hUGT1A1-CATin Fig. 8), yielding $Delta$ HNF1-hUGT1A1-CATplasmid.

Preparation of Nuclear and Whole-Cell Extracts (WCEs). Nuclear extracts from mouse liver were prepared as described (Dignam et al., 1983). Briefly, the final suspension buffer containing20 mM HEPES (pH 7.9), 20 mM KCl, 2 mM MgCl₂, 0.2 mM EDTA, 0.5mM DTT, 20% glycerol, and protease inhibitors (Complete; BoehringerMannheim) was aliquoted, frozen in liquid nitrogen, and storedat $-$ 70°C. WCE was prepared from transfected and nontransfectedhuman embryonic kidney (HEK) 293 cells by disrupting the cellmembrane with three steps of freezing/thawing. The residual debriswere pelleted by centrifugation for 10 min at 12,000g at 4°C.The extracts were aliquoted and stored at $-$ 70°C.

DNase I Footprint Analysis. The DNA fragment from $-$ 253 to +81 of the proximal UGT1A1 promoter sequence was subcloned into the pBLCAT3 vector. This plasmidpossesses restriction sites to generate probes, with either thecoding or noncoding strands labeled. End-labeled DNA fragments(3 × 10⁴ cpm) were incubated with 10 to 50 µg of mouse liver nuclear extracts(MLNEs) or with 10 µg of whole HEK293 cell extracts, and whenindicated, a 100-fold molar excess of oligonucleotide competitorwas added. After 30 min of incubation on ice, the mixtures weredigested with 1.5 U of RQ1DNase I (Promega, Madison, WI) for 1min at room temperature. The reaction was stopped by additionof 200 µl of 50 mM Tris-HCl (pH 8.0), 10 mM EDTA, 2% SDS, 0.4mg/ml proteinase K, and 100 µg/ml glycogen. Samples were separatedon a 7 M urea, 8% polyacrylamide-1× Tris-borate-EDTA sequencinggel. The position of specific DNase I-protected fragments wasdetermined by chemical sequencing of the probe (Maxam and Gilbert,1977).

Electrophoretic Mobility-Shift Assay (EMSA). EMSAs were performed as described (Ijpenberg et al., 1997) with either 10 µg of MLNEs or 2.5 µg of whole HEK293 cell extracts.For supershift experiments, 1 µl of HNF1 $alpha$ -specific antibody wasused. Competition assays were performed by adding a 100-fold excessof unlabeled double-stranded oligonucleotide to the reaction 10min before the addition of labeledprobe.

Cell Culture and Transfection. HEK293 cells were seeded at 3 × 10⁵ cells/well in six-well plates, cultured overnight, and transfected with plasmid DNAs bythe calcium phosphate-DNA coprecipitation method (Jordan et al.,1996). The reporter deletion constructs were at 250 ng/well, andexpression plasmids for HNF1 $alpha$ (pRSV-HNF1 $alpha$ ) and HNF1 $beta$ (pRSV-HNF1 $beta$ )were each at 500 ng/well. Cytomegalovirus- $beta$ -galactosidase expressionvector (50 ng/well; Stratagene, Basel, Switzerland) was includedas an internal standard for transfection efficiency. After 12h, the DNA precipitates were removed, and the cells were furtherincubated in fresh culture medium for 24 h. The CAT activity wasassayed using ¹⁴C-labeled chloramphenicol (Amersham Pharmacia Biotech, Dübendorf,Switzerland) and n-butyryl coenzyme A substrates. The $beta$ -galactosidaseactivity was determined as described (Sambrook et al., 1989).All transfections were performed in duplicate. Activities reportedare an average ± S.D. of three independentexperiments.

	Results

Top Summary Introduction Experimental Procedures Results Discussion References

Cloning of the Mouse UGT1A1 Gene. A mouse genomic DNA library was screened using two oligonucleotides derived from the previously reported mouse UGT1A1 cDNA(Chu et al., 1997). Two clones ( $lambda$ mPGT1A1-1, $lambda$ mPGT1A1-2) were isolatedand characterized (Fig. 1). Together, they form a contig of about25 kb, but only clone $lambda$ mPGT1A1-1 (19-kb insert) contains the entiregene, including several kb of 5'- and 3'-flanking sequences. The5'-end of clone $lambda$ mPGT1A1-2 (20-kb insert) lies within the isoformspecific exon 1A1. This cloned genomic DNA fragment also containsall common exons and extends far into the 3'-flanking region ofthe gene. The common exons 2, 3, 4, and 5 of the UGT1 locus arelocalized about 2 kb downstream of exon 1A1, and their positionrelative to each other as determined by PCR analysis (Fig. 1)is similar to that observed in rat and human (Ritter et al., 1992;Emi et al., 1995).

View larger version (9K):
[in this window]
[in a new window]

Fig. 1. Structure of the mouse UGT1A1 locus. Schematic representation of the mouse UGT1A1 gene deduced from the characterization of the two genomic DNA clones $lambda$ mPGT1A1-1 and $lambda$ mPGT1A1-2 that are shown. Restriction enzyme cleavage sites were mapped only in the region given in bold. The position of the exons was determined by restriction enzyme mapping and PCR analysis of both clones. Only the $lambda$ mPGT1A1-1 clone contains the entire gene with the complete isoform-specific exon 1A1 and promoter sequences. X, XbaI; S, StuI; E, EcoRI; B, BamHI.

A 2.4-kb XbaI restriction fragment from the $lambda$ mPGT1A1-1 clone, which contains exon 1A1 and its 5'-flanking region, was subclonedand sequenced. The insert is 2424 bp long, with 1075 bp of 5'-flankingregion, 904 bp of exon 1A1 sequence, and 445 bp of intron I. Thecoding region of exon 1A1 is 99% identical in terms of amino acidsto that of the reported cloned mouse cDNA (Y $right-arrow$ S change at position25; Chu et al., 1997

). Surprisingly, the 5'-untranslated region(UTR) sequence of this previously reported cDNA is completelydifferent from that of our genomic subclone. To clarify this pointand to determine the real 5'-UTR upstream of the ATG translationstart codon in exon 1A1, we screened a 15-day-old mouse embryoniccDNA library and an adult mouse liver cDNA library using the sameprocedure as for the genomic screening. All 11 independent clonesobtained in this experiment had a 5'-UTR sequence matching thatof the genomic subclone, albeit of different length, reflectingmost likely incomplete cDNA 5'-extension. The 5'-end nucleotideof these cDNAs is indicated in Fig. 2A. The reason for the 5'-UTRstructural discrepancy between our 11 cDNA clones and the previouslyreported clone remains unclear.

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

Fig. 2. Determination of the transcription start sites of the mouse liver UGT1A1 gene. A, sequence of the 5'-UTR of the UGT1A1 gene with the transcription initiation sites (T1, T2, *) and the position of the 5'-end of 11 cDNA clones (vertical arrows). B, primer extension analysis was carried out at three different temperatures using a ³²P-end-labeled primer complementary to nucleotides +95/+120 of the UGT1A1 exon annealed to either 50 µg of total mouse liver RNA (lanes 2-4) or yeast tRNA as a control (lane 1). The primer-extended products were analyzed on an 8% denaturing polyacrylamide gel in parallel with sequencing reactions (lanes 5-8) carried out on the genomic subclone using the same primer as above. Arrows indicate the extended products. T1 and T2 indicate the major and minor transcription initiation site, respectively; Short-stop, prematurely ended extension products (see Results). C, RNase protection assay using an antisense riboprobe corresponding to nucleotides $-$ 76/+336 of the UGT1A1 gene annealed to 20 µg of total mouse liver RNA (lane 5) or yeast tRNA (lane 6) as control. After RNase digestion, protected fragments were resolved on an 8% polyacrylamide gel together with sequencing reactions (lanes 1-4). T1, T2, and * indicate the major, minor, and weak transcription initiation site, respectively. In positioning these initiation sites on the sequencing ladder, a correction of 1 base has been made because of the lower mobility of RNA than DNA of the same length (Sambrook et al., 1989

). The open arrow indicates residual nondigested riboprobe.

Determination of the Mouse UGT1A1 Transcription Start Site. The transcription start site of the mouse UGT1A1 gene was identified by primer extension and RNase protection assays. Primerextension using mouse liver RNA as template was performed at 42,44, and 46°C (Fig. 2B). Three extension products were obtainedin different relative amounts, depending on the reaction temperature.The upstream end of the short-stop product is in the coding sequencein a region with potential secondary structure, which explainsa decrease in the amount of this product at higher temperaturein favor of the longer extension products. The upstream end ofthese latter products is 34 and 38 bp upstream of the ATG translationstart codon at sites we named T1 and T2, respectively. T1 is consideredthe major transcription start site (+1) because it appears strongerthan T2 at all three temperatures used in the extension assay(see Fig. 3A). The 5'-end of the longest cDNA clone we have obtainedis three nucleotides upstream of T2 and most likely correspondsto a minor transcription start site. To confirm the position oftranscription initiation, we carried out RNase protection analysiswith mouse liver RNA and a radiolabeled antisense riboprobe, whichcorresponds to the region between nucleotides $-$ 76 and +336 withrespect to the major transcription start site T1. The protectedfragments also indicate transcriptional start sites at positionsT1 and T2 (Fig. 2C). The bands between these positions in Fig.2C most likely reflect an incomplete digestion of the riboprobe-RNAduplexes (as indicated by the presence of residual nondigestedriboprobe; open arrow). A minor fragment indicating the same startsite as that of the longer cDNA clone could be seen after longerexposure (* in Fig. 2, A and C). All three initiation start sites(*, T1, T2) are shown with respect to the 5'-ends of the 11 cDNAclones mentioned above (Fig. 2A) and in the context of the promotersequence in Fig. 3A.

View larger version (30K):
[in this window]
[in a new window]

Fig. 3. Characteristics of the mouse and human UGT1A1 promoter. A, nucleotide sequence of the mouse UGT1A1 promoter. Nucleotides are numbered with respect to the major transcription start site as determined herein (T1). The minor and a very weak transcription start sites are indicated with a small arrow (T2) and an asterisk, respectively. The translation-initiation codon ATG is boxed, and the first eight amino acids are given. The nucleotide sequence corresponding to the L1 retrotransposon element is indicated in italics. Footprinted regions A, B, C, and D obtained in Fig. 4 are indicated in bold letters. B, comparison of human (Brierley et al., 1996

) and mouse UGT1A1 promoter sequences. The human UGT1A1 nucleotide sequence (top) was aligned with its mouse counterpart (bottom) using the Gap program from the GCG package (Wisconsin Package Version 9.1; Genetics Computer Group, Madison, WI). The transcription initiation site (T1) of the mouse gene and the conserved HNF1 and Sp1 sites are indicated on both mouse and human sequence. The putative human TATA box is indicated. The transcription-initiation site of the human promoter (open arrow) has been determined previously (Ritter et al., 1992

Structural Features of the Mouse UGT1A1 TATA-Less Promoter. Analysis of the promoter region of the mouse UGT1A1 gene revealed several structural features of interest, some of them highlightedfor comparison with the human sequence (Fig. 3, A and B). Themouse promoter has neither a TATA box (Matsui et al., 1980) noran identifiable initiator-type sequence, often found in eukaryoticTATA-less promoters at the transcription start site (Emami etal., 1998). In contrast, the human promoter has a TATA box-likeelement associated with the polymorphic TA repeat responsiblefor some of the cases of Gilbert's disease (Clarke et al., 1997).Otherwise, this TATA box has not yet been characterizedfunctionally.

In addition to this particular feature, an L1 retrotransposon element (Smit et al., 1995

) is present starting at position $-$ 480 in the mouse promoter (Fig. 3A). This insertion was confirmedby PCR analysis and Southern blot of uncloned mouse genomic DNA,which excludes a possible cloning artifact in clone $lambda$ mPGT1A1-1(data not shown). Such an element is absent in the human promoter.Between the human and mouse promoter, there are two conservedregions within the 170 bp upstream of the transcription-initiationsite corresponding to HNF1- and Sp1-binding sites (Fig. 3B). Wethus concentrated on the function of these elements in the regulationof the UGT1A1promoter.

Liver Nuclear Proteins Bind to the Mouse UGT1A1 Promoter. UGT1A1 has a major detoxification function in the liver; therefore, it was of interest to test whether a factor present inMLNEs is able to bind to the putative HNF1 and Sp1 sites describedabove. For this purpose, we performed a DNase I footprinting analysis.As shown in Fig. 4, a total of four independent protected areas,designated A to D, were identified in the proximal promoter region( $-$ 253/+81; noncoding strand). Footprints A (+32/+41) and B ( $-$ 20/+24)are close to and comprise the transcription initiation site, respectively;they are separated by DNase I-hypersensitive sites (*). It isreasonable to speculate that these footprints result from thebinding of factors belonging to the machinery responsible fortranscription initiation, and therefore they were not furthercharacterized herein. Footprint C ( $-$ 68/ $-$ 40) corresponds to theputative HNF1 recognition site and footprinted region D betweennucleotides $-$ 145 to $-$ 122, comprising the putative Sp1 site towhich purified Sp1 can indeed bind in gel-retardation assays,as will be shown later. The same results were obtained with thecoding strand (data not shown). These data, together with theobservation that these binding sites are well conserved in themouse and human promoters, suggested that these factors may playa role in UGT1A1 regulation.

View larger version (47K):
[in this window]
[in a new window]

Fig. 4. Liver nuclear protein-binding sites within the mouse UGT1A1 promoter. DNase I footprinting experiment carried out with a $-$ 253/+81-proximal UGT1A1 promoter fragment (noncoding strand) and increasing amounts of MLNEs. $-$ , DNase I digestion of the probe without added protein; +, DNase I digestion of the probe with 50 µg of purified bovine serum-albumin. Amounts of nuclear extracts used are 10 µg (lane 5), 20 µg (lane 6), 30 µg (lane 7), and 40 µg (lane 8). Protected areas are indicated on the right of the autoradiogram. DNase I-hypersensitive sites present between the A and B regions are indicated by *. Also shown are chemical sequencing ladders G and G+A (lanes 1 and 2).

The Mouse UGT1A1 Promoter Is Transactivated by HNF1. The functional role of HNF1 was assayed by cotransfection assays performed with HNF1 $alpha$ and HNF1 $beta$ expression vectors and a CATreporter gene driven by the mouse UGT1A1 promoter comprising decreasinglengths of 5'-upstream sequences ( $-$ 1074/+19, $-$ 93/+19, $-$ 44/+19).The empty expression vector (Rous sarcoma virus) and promoterlessreporter CAT vector (pBLCAT3) were used as controls. The recipientcells were the HEK293 cells in which HNF1 cannot be detected.The results show that both HNF1 $alpha$ and HNF1 $beta$ are able to transactivateboth the $-$ 1074/+19 mUGT1A1-CAT reporter gene and the $-$ 93/+19 mUGT1A1-CATconstruct, both of which contain the HNF1 site (Fig. 5). The minimalpromoter $-$ 44/+19 still has a relatively high basal promoter activity,a noteworthy feature for a TATA-less promoter. Some residual HNF1-dependentstimulatory activity was seen with this minimal promoter thatis thought to be due to vector sequences brought close to thepromoter as a result of upstream promoter deletion (see resultswith the promoterless CAT-vector). Instead of analyzing this effectfurther, we performed site-directed mutagenesis of the HNF1 sitein the context of a relatively large promoter region ( $-$ 455/+19).A complete loss of HNF1-dependent stimulation of the mutated promoterconfirmed that the HNF1 element is responsible for mediating inductionby the liver-enriched transcription factor (Fig. 5, $Delta$ HNF1-mUGT1A1-CAT).We conclude that HNF1 is a transactivator of the UGT1A1 gene andthat the stimulatory effect is mediated by the HNF1 binding sitelocated at $-$ 68/ $-$ 40. It is noteworthy that removal of L1 elementsequences did not influence HNF1 responsiveness.

View larger version (12K):
[in this window]
[in a new window]

Fig. 5. HNF1 $alpha$ and HNF1 $beta$ transactivate the mouse UGT1A1 promoter. HEK293 cells were cotransfected in six-well plates with 0.25 µg per well of the different deletion and mutant reporter constructs and 0.5 µg of expression vector for HNF1 $alpha$ (RSV-HNF1 $alpha$ ), HNF1 $beta$ (RSV-HNF1 $beta$ ), or empty vector (RSV) as a control. A pCMV $beta$ -galactosidase (50 ng per well) expression vector was included as an internal control of transfection efficiency. Results are the mean of at least three independent experiments ± S.D. Deletion constructs are depicted, with the L1 element indicated as a black bar, and the position of the Sp1 and HNF1 sites are given according to the results of Fig. 4. In $Delta$ HNF1-mUGT1A1-CAT, the mutated HNF1 site is represented by a cross; this result is taken from Fig. 8. pBLCAT3 was used as a promoterless control reporter gene.

HNF1 Binds to the UGT1A1 Promoter. To assess whether the HNF1-mediated transactivation is due to a direct binding of the factor to the HNF1-binding site in thepromoter, as suggested by the results presented above, we carriedout EMSAs using the UGT1A1-HNF1 site as a probe. We first confirmedthat a factor in the MLNE binds to this site, as shown previouslyby the DNase I footprinting experiment. A major retarded complex(C1) was detected in the presence of the nuclear extract (Fig.6A, lane 2). This complex was competed away by a molar excessof a HNF1-specific oligonucleotide added to the binding reaction(lane 5), whereas binding sites for other transcription factorswere unable to displace the complex (lanes 3, 4, 6, and 7). Wealso observed a faster-migrating minor complex (C2). This C2 complexmost likely contains HNF3, because it was specifically displacedby a molar excess of HNF3 sites, which is in accordance with previouslyreported results indicating that HNF3 may bind to HNF1 sites (Gregoriet al., 1993). Figure 6B shows that the C1 complex was disruptedby a polyclonal antibody directed against HNF1 $alpha$ (lane 3), allowinga reinforcement of C2 complex formation. The nonspecific bandobserved with the antibody alone (lane 4) has been previouslyreported (Chouard et al., 1997). Together, these results providestrong evidence that C1 is due to the occupancy of the UGT1A1-HNF1site by HNF1 $alpha$ , which is abundant in liver (Rey-Campos et al.,1991).

View larger version (41K):
[in this window]
[in a new window]

Fig. 6. HNF1 proteins bind to the C site of the mouse UGT1A1 promoter. A, EMSA experiments using a MLNE were performed with a radiolabeled oligonucleotide corresponding to site C (HNF1-binding site) of the UGT1A1 promoter in the presence or absence of a 100-fold excess of different competitor oligonucleotides as indicated at the top of the autoradiogram. For the identification of C1 and C2 complexes, see text. * is an unspecific band. B, supershift experiments in which EMSA with the radiolabeled site C oligonucleotide was carried out with MLNE in the presence or absence of a specific antibody directed against HNF1 $alpha$ (Chouard et al., 1997

). * is an unspecific band, as in A. ** is an unspecific band generated by the antibody, as described (Chouard et al., 1997

). C, sequence of the different wild-type and mutated HNF1-binding sites comprised in the oligonucleotides used in EMSA, as compared with the consensus HNF1-binding site. Nucleotides corresponding to the consensus binding site are underlined in ALB-HNF1, UGT1A1-HNF1, and mut UGT1A1-HNF1. The matching index is given in brackets. D, EMSA using overexpressed HNF1 $alpha$ or HNF1 $beta$ in HEK293 cells was performed with radiolabeled site C as probe (see above) in the presence of 100- or 500-fold excess of mutant site C (mutUGT1A1) or wild-type site C (UGT1A1) competitor oligonucleotides.

To strengthen the evidence for specific binding of HNF1 $alpha$ , we used the mutated UGT1A1-HNF1 site depicted in Fig. 6C as competitor.Figure 6D shows that a 100- and 500-fold molar excess of the mutantoligonucleotide was unable to displace the HNF1 $alpha$ -retarded complexes(lanes 4 and5).

Finally, we have demonstrated that HNF1 $beta$ is also able to bind this element, as suggested by the transfection result shownin Fig. 5. Indeed, overexpressed HNF1 $beta$ binds to the UGT1A1-HNF1site (Fig. 6D, lane 6). The complex is displaced by a 100- and500-fold molar excess of the probe (lanes 7 and 8) but not bythe mutant oligonucleotide (lanes 9 and 10). Altogether, theseresults provide evidence for a specific interaction of HNF1 withthe UGT1A1 promoter at a site that we demonstrated to be responsiblefor the transcriptional activation mediated by this transcriptionfactor.

HNF1 and Sp1 Do Not Cooperate for the Control of the UGT1A1 Promoter. The footprinting experiment using MLNEs revealed a binding site for Sp1 in the mouse UGT1A1 promoter, which is conserved inthe human promoter, 54 bp upstream of the HNF1 site. This observationwas confirmed in EMSA experiments with whole HEK293 cell extractsas well as with purified Sp1 for both the mouse and human Sp1sites (data notshown).

The proximity of HNF1- and Sp1-binding sites on the UGT1A1 promoter prompted us to test whether the binding of the two factorswas independent or cooperative. Indeed, it has been observed thatSp1 can bind cooperatively to DNA with transcription factors suchas C/EBP $alpha$ (Lee et al., 1994

). For this purpose, we carried outoligonucleotide competition in DNase I footprint experiments usingMLNEs or whole HEK293 cell extracts from cells transfected witheither HNF1 $alpha$ or HNF1 $beta$ as well as mock-transfected cell extractsas control. HEK293 cells contain sufficient amounts of endogenousSp1-binding activity to produce a footprint over the UGT1A1-Sp1site (Fig. 7, lanes 9, 13, and 17). Competitive inhibition ofbinding to the Sp1 site did not influence binding to the HNF1site (lanes 7, 15, and 19). Similarly, competitive inhibitionof binding to the HNF1 site did not affect protein interactionwith the Sp1 site (lanes 6, 14, and 18). Competition with an unrelatedcontrol oligonucleotide (lanes 8, 16, and 20) had no effects oneither of these two sites. These results indicate that, in thisassay, binding of HNF1 on the promoter occurs independently ofSp1 binding.

View larger version (98K):
[in this window]
[in a new window]

Fig. 7. Noncooperative binding between Sp1 and HNF1 within the proximal mouse UGT1A1 promoter. DNase I footprinting was carried out using a $-$ 253/+81 UGT1A1 promoter fragment (noncoding strand) and protein extracts from mouse liver and HEK293 cells as indicated at the top of the gel in the presence of 100-fold excess of different competitor oligonucleotides. Mock, WCE from mock-transfected HEK293 cells; HNF1 $alpha$ , WCE from HNF1 $alpha$ -transfected HEK293 cells; HNF1 $beta$ , WCE from HNF1 $beta$ -transfected HEK293 cells. $-$ , DNase I digestion of the probe without added protein; +, DNase I digestion of the probe with 50 µg of purified BSA; H, HNF1 consensus oligonucleotide; S, Sp1 consensus; C, C/EBP consensus oligonucleotide. Protected areas corresponding to the Sp1- and HNF1-binding sites are indicated on the right of the gel. The sequencing ladder tracks G and G+A are indicated.

The fact that cooperative binding to the HNF1 and Sp1 sites could not be detected in competition footprinting experimentsdoes not necessarily preclude functional interaction between thetwo proteins during transcriptional stimulation. This kind offunctional cooperation has indeed been demonstrated between Sp1and nuclear hormone receptors (Krey et al., 1995

). To test thispossibility, cotransfection experiments were performed using amouse promoter construct mutated at either the Sp1 site ( $Delta$ Sp1-mUGT1A1-CAT)or HNF1 site ( $Delta$ HNF1-mUGT1A1-CAT). The mutation introduced in theHNF1 site corresponds to that shown previously in Fig. 6C (mutUGT1A1),which hinders HNF1 binding. The wild-type promoter or the promotersimultaneously mutated at the two sites under analysis ( $Delta$ HNF1/Sp1-mUGT1A1-CAT)were used as positive and negative controls, respectively. Asshown previously, invalidation of the HNF1 site abolished transcriptionalactivation of the promoter by HNF1, whereas mutation of the Sp1site had no effect on transactivation by HNF1 (Fig. 8). This indicatesthat there is no functional interaction between the Sp1 and HNF1sites in our experimental system. However, mutation of the Sp1-bindingsite alone reduced strongly the basal activity of the promoterin absence of cotransfected HNF1. This observation suggests thatSp1 plays a role in the basal activity of the mouse UGT1A1 promoter.Because the human and mouse UGT1A1 promoters display a very wellconserved HNF1 site, we tested whether HNF1 is able to mediatetransactivation of the human promoter. As shown in Fig. 8, thebasal activity of the human promoter ( $-$ 617 to +15) is similarto its mouse counterpart in HEK293 cells. HNF1 $alpha$ and HNF1 $beta$ activatedthe human UGT1A1 promoter even more strongly than the mouse promoter.Similarly to what has been observed with the mouse promoter, disruptionof the HNF1 binding site ( $Delta$ HNF1-hUGT1A1-CAT) abolished HNF1-mediatedtransactivation. In conclusion, both the mouse and human UGT1A1promoters can be transcriptionally regulated by HNF1 transcriptionfactors, despite important structural differences between them.

View larger version (14K):
[in this window]
[in a new window]

Fig. 8. Absence of functional interaction between HNF1 $alpha$ and Sp1 in transactivation of the mouse UGT1A1 promoter. HEK293 cells were cotransfected in six-well plates with 0.25 µg per well of different mutant reporter constructs and 0.5 µg of expression vector for HNF1 $alpha$ (RSV-HNF1 $alpha$ ), HNF1 $beta$ (RSV-HNF1 $beta$ ), or empty vector as control (RSV). A pCMV $beta$ -galactosidase (50 ng per well) expression vector was included as an internal control for transfection efficiency. Results are the mean of at least three independent experiments ± S.D. The reporter constructs used are depicted; mutated Sp1, and HNF1 sites are indicated by a cross. pBLCAT3 was used as promoterless control reporter.

	Discussion

Top Summary Introduction Experimental Procedures Results Discussion References

Glucuronidation of bilirubin is essential for its excretion from the liver into the bile. In human, UGT1A1 is the major UGTisoform involved in this process (Bosma et al., 1994). Consequently,alteration in UGT1A1 gene expression or mutations in the codingregion of this gene can lead to a complete or partial absenceof bilirubin glucuronidation activity, which results in toxicaccumulation of unconjugated bilirubin (Hauser and Gollan, 1990).One of the ways to study and better understand bilirubin metabolismin human is to compare it to other mammalian species, such asthe increasingly used mouse model. For this purpose, we have clonedand functionally characterized the mouse UGT1A1 promoter. Importantstructural differences with the human promoter were found. Surprisingly,the mouse UGT1A1 promoter is TATA-less and consequently does notcontain any of the TA repeats found in human. In contrast, bothhuman and mouse promoter activities are stimulated by HNF1 $alpha$ andHNF1 $beta$ via a functional HNF1 site particularly well conserved betweenthe twopromoters.

The Mouse UGT1A1 Promoter Lacks a TATA Box. Two major new features occur only in the mouse UGT1A1 promoter in comparison to the human promoter. First, the mouse UGT1A1promoter has no apparent TATA box, as observed previously forthe rat UGT1A7 promoter (Metz and Ritter, 1998). In contrast,other UGTs belonging to family 1 (Emi et al., 1996) as well asto family 2 (Mackenzie and Rodbourn, 1990) possess a TATA-likeelement, indicating that there is no common promoter structurefor all UGT isoforms. It is noteworthy that the rat UGT1A7 promoterhas multiple transcription start sites clustered within 45 bp,whereas the mouse UGT1A1 has only two independent well detectabletranscription start sites clustered in less than 10 bp, whichcan be detected by analysis of liver transcripts. Despite thelack of a TATA-binding protein binding site, it is clear thatthe mouse UGT1A1 transcriptional start site is well defined, suggestingthat binding of transcription factors to this promoter directlyinteracts with the basal transcription machinery to help in positioningRNA polymerase II. HNF1 indeed is one of the transcription factorsthat have been shown to interact directly with components of thegeneral transcription apparatus, such as transcription factorIID or transcription factor IIB (Ktistaki and Talianidis, 1997).The second characteristic feature of the mouse promoter is thepresence of a retrotransposon-like sequence element, which belongsto the L1 family, at 480 bp upstream the transcription start site.The L1 element is found at more than 100,000 copies in mouse andrepresents about 10% of the genome (Smit et al., 1995). However,the majority of the L1 elements are truncated and not active intransposition (Kolosha and Martin, 1995). This is the case forthe element identified in the mouse UGT1A1 promoter because itslacks the 5'-long terminal repeat. The recent characterizationof the apolipoprotein(a) enhancer in mouse, which resides withina L1 element, illustrates the possibility of a regulatory actionof these elements on neighboring promoters (Yang et al., 1998).However, further studies are needed, especially in hepatocytesrather than in HEK293 cells, to evaluate the relevance, if any,of this L1 element insertion for tissue-specific activity of themouse UGT1A1gene.

HNF1 Binds to and Activates the Mouse UGT1A1 Promoter. We have demonstrated that both HNF1 $alpha$ and HNF1 $beta$ bind to the mouse UGT1A1 promoter and are able to transactivate it. However,because HNF1 $beta$ is less expressed in adult mouse liver than HNF1 $alpha$ ,it is very likely that it is the latter factor that plays a regulatoryrole in this organ. Our results suggest that HNF3 also binds tothe HNF1 site, although the signal of HNF1 is much stronger thanthat of HNF3 in liver nuclear extracts. It will be interestingto investigate whether there is a competition between these twofactors relevant for expression of this gene in liver. The HNF1-bindingsite of the mouse UGT1A1 promoter is very similar to that of therat albumin promoter, which displays a very well conserved half-siteand a more divergent one with respect to the consensus sequence(Cereghini, 1996). Consistent with previous studies on the albumin-HNF1site, HNF1 proteins failed to bind and transactivate the mouseUGT1A1 promoter when the conserved half-site is mutated. Our studyprovides strong evidence for HNF1 $alpha$ and HNF1 $beta$ being involved inthe expression of this member of the UGT superfamily in rodents.In adult mouse, HNF1 $alpha$ and HNF1 $beta$ are expressed in the same tissues(kidney, liver, intestine, and pancreas; Rey-Campos et al., 1991)but at different relative levels. In liver, HNF1 $beta$ is less expressedthan HNF1 $alpha$ , whereas both are present at similar levels in kidney.This pattern of expression correlates with that of the rat UGT1A1,which is predominantly found in liver, and less in kidney (Emiet al., 1995). Furthermore, HNF1 $alpha$ and HNF1 $beta$ play an importantrole during development. It has been shown that HNF1 $beta$ , which systematicallyprecedes HNF1 $alpha$ expression, is involved in early events of liverand kidney morphogenesis, whereas HNF1 $alpha$ is required for maintenanceof the differentiated state (Cereghini, 1996). Further studiesare required to elucidate to what extent these two factors contributeto the developmental expression of the UGT1A1 gene inmouse.

Is HNF1 Crucial for the UGT1A1 Gene Expression in Human and Mouse? The structural differences between human and mouse UGT1A1 promoters raised the question as to whether they are subjected tothe same regulatory process. Comparison of the two promoters revealedconserved HNF1- and Sp1-binding sites, and our study also indicatesthat HNF1 $alpha$ and HNF1 $beta$ transactivate both the human and mouse UGT1A1promoter in the same manner. However, an extrapolation from cellculture experiments to the in vivo situation in human is not possiblewithout further consideration. For instance, neither bilirubinglucuronidation nor UGT1A1 mRNA can be detected in human kidney(McGurk et al., 1998) in which HNF1 proteins are expressed andactive. This indicates that HNF1 is not sufficient for the humanUGT1A1 expression in thisorgan.

Recent studies using the knockout technology have revealed a role of hepatic transcription factors in mouse UGT1A1 expression.The inactivation of the HNF1 $alpha$ gene by homologous recombinationresulted in a complex phenotype with impaired functions in liverand kidney (Pontoglio et al., 1996

). The HNF1 $alpha$ $-$ / $-$ mice lack expressionof the HNF1 target gene phenylalanine hydroxylase, whereas theexpression of other HNF1 target genes such as albumin, $alpha$ -antitrypsin,and $alpha$ - and $beta$ -fibrinogen was only partially reduced. Interestingly,these mutant mice exhibit a mild hyperbilirubinemia. Based onthe results reported herein, it is likely that it is caused byan altered expression of the UGT1A1 gene. Furthermore, our resultssuggest that the residual expression of UGT1A1 indicated by themild hyperbilirubinemia might be caused by HNF1 $beta$ , which is expressedin the liver (see above) and is also a transcriptional regulatorof the UGT1A1 promoter. HNF1 $beta$ may partially rescue the HNF1 $alpha$ deficiency,as was proposed for other HNF1-target genes (Pontoglio et al.,1996

). Although this is the most plausible explanation, we cannotexclude the possibility that other bilirubin UGTs isoforms maintainbilirubin glucuronidation in the HNF1 $alpha$ $-$ / $-$ mice.

Often, tissue-enriched factors cooperate with ubiquitous factors, for instance C/EBP $alpha$ with Sp1 (Lee et al., 1994

). Herein,we show that Sp1, which binds upstream of HNF1 on the UGT1A1 promoter,seems to have no influence on HNF1 binding or on its transcriptionalactivity in HEK293 cells. However, we have also demonstrated thatSp1 alters the mouse UGT1A1 promoter activity independently ofHNF1. Further analysis of this promoter, which may identify additionalregulatory factors, is necessary to assess novel interactionsbetween the transcription factors involved in itsregulation.

In conclusion, we have identified HNF1 as the first important transcriptional regulator of UGT1A1 gene expression in mouseand human. It will now be the aim of further studies to determinethe extent of its regulatory contribution in UGT1A1 expressionwith respect to the species- and tissue-specific characteristicsof bilirubinglucuronidation.

	Acknowledgments

We thank M. Yaniv and M. Pontoglio for the kind gift of HNF1 expression plasmids and antibody and G. Lazennec for his helpin DNase I footprint experiments. We also thank A. K. Hihi andD. Robyr for critical reading of the manuscript and for helpfuldiscussions.

	Footnotes

Received January 4, 1999; Accepted May 26, 1999

¹ The nucleotide sequence reported in this paper has been submitted to the GenBank database with GenBank accession number AF093878.

This work was supported by grants from the Swiss National Science Foundation (B.D. and W.W.), the Etat de Vaud, and the ConseilRégional de Bourgogne. P.B. was supported by a fellowship fromthe Association de Recherche sur le Cancer (ARC; Villejuif, France)and the Etat deVaud.

Send reprint requests to: Walter Wahli, Institut de Biologie Animale, Bâtiment de Biologie, Université de Lausanne, CH-1015 Lausanne, Switzerland. E-mail: walter.wahli{at}iba.unil.ch

	Abbreviations

UGT, UDP-glucuronosyltransferases; HEK, human embryonic kidney; EMSA, electrophoretic mobility shift assay; MLNE, mouse liver nuclear extract; PCR, polymerase chain reaction; CAT, chloramphenicol acetyltransferase; UTR, untranslated region, RSV, Rous sarcoma virus; TA, thymidine/adenine; WCE, whole-cell extract.

	References

Top Summary Introduction Experimental Procedures Results Discussion References

Aono S, Adachi Y, Uyama E, Yamada Y, Keino H, Nanno T, Koiwai O and Sato H (1995) Analysis of genes for bilirubin UDP-glucuronosyltransferase in Gilbert's syndrome. Lancet 345: 958-959[Medline].
Beutler E, Gelbart T and Demina A (1998) Racial variability in the UDP-glucuronosyltransferase 1 (UGT1A1) promoter-A balanced polymorphism for regulation of bilirubin metabolism. Proc Natl Acad Sci USA 95: 8170-8174[Abstract/Free Full Text].
Bosma PJ, Chowdhury JR, Bakker C, Gantla S, de Boer A, Oostra BA, Lindhout D, Tytgat GN, Jansen PL, Oude Elferink RP and Chowdhury NR (1995) The genetic basis of the reduced expression of bilirubin UDP-glucuronosyltransferase 1 in Gilbert's syndrome. N Engl J Med 333: 1171-1175[Abstract/Free Full Text].
Bosma PJ, Seppen J, Goldhoorn B, Bakker C, Oude Elferink RP, Chowdhury JR, Chowdhury NR and Jansen PL (1994) Bilirubin UDP-glucuronosyltransferase 1 is the only relevant bilirubin glucuronidating isoform in man. J Biol Chem 269: 17960-17964[Abstract/Free Full Text].
Brierley CH, Senafi SB, Clarke D, Hsu MH, Johnson EF and Burchell B (1996) Regulation of the human bilirubin UDP-glucuronosyltransferase gene. Adv Enzyme Regul 36: 85-97[Medline].
Cereghini S (1996) Liver-enriched transcription factors and hepatocyte differentiation. FASEB J 10: 267-282[Abstract].
Chouard T, Jeannequin O, Rey-Campos J, Yaniv M and Traincard F (1997) A set of polyclonal and monoclonal antibodies reveals major differences in post-translational modification of the rat HNF1 and vHNF1 homeoproteins. Biochimie 79: 707-715[Medline].
Chu Q, Lei W, Gudehithlu K, Matwyshyn GA, Bocchetta M and Kong ANT (1997) cDNA cloning of the mouse bilirubin/phenol family of UDP-glucuronosyltransferase (mugtbr2-like). Pharm Res 14: 662-666[Medline].
Clarke DJ, Moghrabi N, Monaghan G, Cassidy A, Boxer M, Hume R and Burchell B (1997) Genetic defects of the UDP-glucuronosyltransferase-1 (UGT1) gene that cause familial non-haemolytic unconjugated hyperbilirubinaemias. Clin Chim Acta 266: 63-74[Medline].
Dignam JD, Lebovitz RM and Roeder RG (1983) Accurate transcription initiation by RNA polymerase II in a soluble extract from isolated mammalian nuclei. Nucleic Acids Res 11: 1475-1489[Abstract/Free Full Text].
Emami KH, Burke TW and Smale ST (1998) Sp1 activation of a TATA-less promoter requires a species-specific interaction involving transcription factor IID. Nucleic Acids Res 26: 839-846[Abstract/Free Full Text].
Emi Y, Ikushiro S and Iyanagi T (1995) Drug-responsive and tissue-specific alternative expression of multiple first exons in rat UDP-glucuronosyltransferase family 1 (UGT1) gene complex. J Biochem 117: 392-399[Abstract/Free Full Text].
Emi Y, Ikushiro S and Iyanagi T (1996) Xenobiotic responsive element-mediated transcriptional activation in the UDP-glucuronosyltransferase family 1 gene complex. J Biol Chem 271: 3952-3958[Abstract/Free Full Text].
Gregori C, Kahn A and Pichard AL (1993) Competition between transcription factors HNF1 and HNF3, and alternative cell-specific activation by DBP and C/EBP contribute to the regulation of the liver-specific aldolase B promoter. Nucleic Acids Res 21: 897-903[Abstract/Free Full Text].
Hansen AJ, Lee YH, Gonzalez FJ and Mackenzie PI (1997) HNF1 alpha activates the rat UDP glucuronosyltransferase UGT2B1 gene promoter. DNA Cell Biol 16: 207-214[Medline].
Hansen AJ, Lee YH, Sterneck E, Gonzalez FJ and Mackenzie PI (1998) C/EBPalpha is a regulator of the UDP glucuronosyltransferase UGT2B1 gene. Mol Pharmacol 53: 1027-1033[Abstract/Free Full Text].
Hauser SC and Gollan JL (1990) Mechanistic and molecular aspects of hepatic bilirubin glucuronidation. Progress Liver Dis 9: 225-235.
Ijpenberg A, Jeannin E, Wahli W and Desvergne B (1997) Polarity and specific sequence requirements of peroxisome proliferator-activated receptor (PPAR)/retinoid X receptor heterodimer binding to DNA. A functional analysis of the malic enzyme gene PPAR response element. J Biol Chem 272: 20108-20117[Abstract/Free Full Text].
Jansen PL, Mulder GJ, Burchell B and Bock KW (1992) New developments in glucuronidation research: Report of a workshop on "Glucuronidation, its role in health and disease." Hepatology 15: 532-544[Medline].
Jordan M, Schallhorn A and Wurm FM (1996) Transfecting mammalian cells: Optimization of critical parameters affecting calcium-phosphate precipitate formation. Nucleic Acids Res 24: 596-601[Abstract/Free Full Text].
Kolosha VO and Martin SL (1995) Polymorphic sequences encoding the first open reading frame protein from LINE-1 ribonucleoprotein particles. J Biol Chem 270: 2868-2873[Abstract/Free Full Text].
Krey G, Mahfoudi A and Wahli W (1995) Functional interactions of peroxisome proliferator-activated receptor, retinoid-X receptor, and Sp1 in the transcriptional regulation of the acyl-coenzyme-A oxidase promoter. Mol Endocrinol 9: 219-231[Abstract].
Ktistaki E and Talianidis I (1997) Modulation of hepatic gene expression by hepatocyte nuclear factor 1. Science (Wash DC) 277: 109-112[Abstract/Free Full Text].
Lee YH, Sauer B, Johnson PF and Gonzalez FJ (1997) Disruption of the C/EBP-alpha gene in adult mouse liver. Mol Cell Biol 17: 6014-6022[Abstract].
Lee YH, Yano M, Liu SY, Matsunaga E, Johnson PF and Gonzalez FJ (1994) A novel cis-acting element controlling the rat CYP2D5 gene and requiring cooperativity between C/EBP beta and an Sp1 factor. Mol Cell Biol 14: 1383-1394[Abstract/Free Full Text].
Mackenzie PI, Owens IS, Burchell B, Bock KW, Bairoch A, Belanger A, Fournel-Gigleux S, Green M, Hum DW, Iyanagi T, Lancet D, Louisot P, Magdalou J, Chowdhury JR, Ritter JK, Schachter H, Tephly TR, Tipton KF and Nebert DW (1997) The UDP glycosyltransferase gene superfamily: Recommended nomenclature update based on evolutionary divergence. Pharmacogenetics 7: 255-269[Medline].
Mackenzie PI and Rodbourn L (1990) Organization of the rat UDP-glucuronosyltransferase, UDPGTr-2, gene and characterization of its promoter. J Biol Chem 265: 11328-11332[Abstract/Free Full Text].
Matsui T, Segall J, Weil PA and Roeder RG (1980) Multiple factors required for accurate initiation of transcription by purified RNA polymerase II. J Biol Chem 255: 11992-11996[Abstract/Free Full Text].
Maxam AM and Gilbert W (1977) A new method for sequencing DNA. Proc Natl Acad Sci USA 74: 560-564[Abstract/Free Full Text].
McGurk KA, Brierley CH and Burchell B (1998) Drug glucuronidation by human renal UDP-glucuronosyltransferases. Biochem Pharmacol 55: 1005-1012[Medline].
Metz RP and Ritter JK (1998) Transcriptional activation of the UDP-glucuronosyltransferase 1A7 gene in rat liver by aryl hydrocarbon receptor ligands and oltipraz. J Biol Chem 273: 5607-5614[Abstract/Free Full Text].
Pontoglio M, Barra J, Hadchouel M, Doyen A, Kress C, Bach JP, Babinet C and Yaniv M (1996) Hepatocyte nuclear factor 1 inactivation results in hepatic dysfunction, phenylketonuria, and renal Fanconi syndrome. Cell 84: 575-585[Medline].
Rey-Campos J, Chouard T, Yaniv M and Cereghini S (1991) vHNF1 is a homeoprotein that activates transcription and forms heterodimers with HNF1. EMBO J 10: 1445-1457[Medline].
Ritter JK, Chen F, Sheen YY, Tran HM, Kimura S, Yeatman MT and Owens IS (1992) A novel complex locus UGT1 encodes human bilirubin, phenol, and other UDP-glucuronosyltransferase isozymes with identical carboxyl termini. J Biol Chem 267: 3257-3261[Abstract/Free Full Text].
Sambrook J, Fritsch EF and Maniatis T (1989) Molecular Cloning: A Laboratory Manual. Cold Spring Harbor Laboratory Press, Plainview, NY.
Smit AF, Toth G, Riggs AD and Jurka J (1995) Ancestral, mammalian-wide subfamilies of LINE-1 repetitive sequences. J Mol Biol 246: 401-417[Medline].
Strassburg CP, Manns MP and Tukey RH (1998) Expression of the UDP-glucuronosyltransferase 1A locus in human colon $---$ Identification and characterization of the novel extrahepatic UGT1A8. J Biol Chem 273: 8719-8726[Abstract/Free Full Text].
Strassburg CP, Oldhafer K, Manns MP and Tukey RH (1997) Differential expression of the UGT1A locus in human liver, biliary, and gastric tissue $---$ Identification of UGT1A7 and UGT1A10 transcripts in extrahepatic tissue. Mol Pharmacol 52: 212-220[Abstract/Free Full Text].
Yang Z, Boffelli D, Boonmark N, Schwartz K and Lawn R (1998) Apolipoprotein(a) gene enhancer resides within a LINE element. J Biol Chem 273: 891-897[Abstract/Free Full Text].

This article has been cited by other articles:

H. I. Sims, C. B. Baughman, and G. R. Schnitzler
Human SWI/SNF directs sequence-specific chromatin changes on promoter polynucleosomes
Nucleic Acids Res., November 1, 2008; 36(19): 6118 - 6131.
[Abstract] [Full Text] [PDF]

D. A. Gardner-Stephen and P. I. Mackenzie
Isolation of the UDP-Glucuronosyltransferase 1A3 and 1A4 Proximal Promoters and Characterization of Their Dependence on the Transcription Factor Hepatocyte Nuclear Factor 1{alpha}
Drug Metab. Dispos., January 1, 2007; 35(1): 116 - 120.
[Abstract] [Full Text]

Activation of the Mouse TATA-less and Human TATA-Containing UDP-Glucuronosyltransferase 1A1 Promoters by Hepatocyte Nuclear Factor 11

Activation of the Mouse TATA-less and Human TATA-Containing UDP-Glucuronosyltransferase 1A1 Promoters by Hepatocyte Nuclear Factor 1¹