The Role of Sp1 and AP-2 in Basal and Protein Kinase A-induced Expression of Mitochondrial Serine:Pyruvate Aminotransferase in Hepatocytes

doi:10.1074/jbc.M201380200

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The Role of Sp1 and AP-2 in Basal and Protein Kinase A-induced Expression of Mitochondrial Serine:Pyruvate Aminotransferase in Hepatocytes^*

Chiharu Uchida^§, Toshiaki Oda, Tsuyoshi Sugiyama^¶, Sunao Otani, Masatoshi Kitagawa, and Arata Ichiyama

From the Department of Biochemistry I and Department of ^¶ Internal Medicine III, Hamamatsu University School of Medicine, 1-20-1 Hamamatsu, Shizuoka, Japan

Received for publication, February 11, 2002, and in revised form, July 9, 2002

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Transcription of mitochondrial serine:pyruvate aminotransferase (SPT) mRNA (SPTm-mRNA) in rat liver is unique in that it occursfrom the upstream site of the two transcription start sites withinthe first exon of the SPT gene and is selectively enhanced bycAMP via the protein kinase A (PKA) signaling pathway. In thisstudy, we identified the DNA elements and nuclear factors responsiblefor the basal and PKA-induced activities of the upstream promoter.By using a luciferase reporter assay with HepG2 cells, DNase Ifootprinting analysis, and gel shift experiments, we identifiedthe binding sites for Sp1 and AP-2 within the regions $-$ 125 to $-$ 89 and $-$ 14 to +10, respectively. Mutational analyses indicatedthat these regions are essential for the transcription factorbinding and the SPT promoter activity. Expression of AP-2 causeda marked increase in the basal promoter activity to about thesame level as that achieved by PKA. On the other hand, both thebasal and PKA-induced activities were elevated by overexpressionof Sp1, its effect on PKA-induced activity being more pronouncedwith coexpression of CBP and repressed by E1A oncoprotein. Theseresults suggest that AP-2 and Sp1 regulate basal promoter activity,and Sp1 is also involved in PKA-mediated expression of the ratSPT gene in concert with the transcriptional coactivator CBP.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Serine:pyruvate aminotransferase (SPT¹; alternatively named alanine:glyoxylate aminotransferase-1) is a liver-specific enzyme,and a bipartite transcription initiation mechanism is involvedin its expression in the rat liver. Use of the upstream transcriptionstart site (+1) results in production of mitochondrial SPT mRNA(SPTm-mRNA) in response to a rise in intracellular cAMP level,whereas the downstream transcription start site (+66) is responsiblefor continuous generation of peroxisomal SPT mRNA (SPTp-mRNA)without notable induction by stimulants (1-3). These two mRNAsdiffer from each other in the lengths of 5'-terminal sequences(2, 4). SPTm-mRNA is 65 bases longer than SPTp-mRNA andhas an extra 5' sequence that encodes an N-terminal mitochondria-targetingsignal, whereas SPTp-mRNA lacks this sequence and the translatedproduct is translocated into peroxisomes, presumably being directedby an intramolecular peroxisomal targeting sequence (5-9). Thus,the unique feature of this gene is that the alternative usageof two transcription start sites eventually determines organellelocalization of the expressionproduct.

The 5'-sequences of the SPT genes are well conserved up to 25-28 bp upstream from the downstream start sites, but the upperregion is relatively diverse among different animal species (10-12).Our previous studies showed that SPT is involved in both serineand glyoxylate metabolism (13, 14). The role of SPT in glyoxylatemetabolism is important, because glyoxylate can be oxidized tooxalate, a useless and toxic end product of metabolism, unlessit is efficiently metabolized to glycine. The major pathways ofhepatic glyoxylate production in herbivores and carnivores seemto be oxidation of glycolate in peroxisomes and metabolism ofhydroxyproline in mitochondria, respectively (15). Therefore,it is important that the organelle localization of SPT is foodhabit-dependent. The marmoset, like the rat (16), has SPT inboth of the organelles in the liver (12). Carnivores, such ascats and dogs, have the enzyme largely in mitochondria, whereasit is located entirely in peroxisomes in herbivores and man (10,17). As for cat SPT, Lumb et al. (10) showed that transcriptionof the gene occurred almost entirely from a site correspondingto the upstream start site in the rat SPT gene, consistent withmitochondrial localization. In the human and rabbit SPT genes,the transcription start site is also a site corresponding to theupstream site in the rat gene, but the first ATG codon for translationof the N-terminal mitochondria-targeting signal in these speciesis mutated to ACA or AUA (11-12). Therefore, the methionine codonfirst encountered in translation should be the downstream AUGthat corresponds to the N-terminal methionine of SPT (18). Inthe case of the rat and marmoset, it seems that the downstreamstart site had been prepared to distribute SPT to peroxisomesin addition to mitochondria to adapt their metabolism to theiromnivorous food habits. Thus, regulation of transcription of theSPT gene is closely linked to its specific organelle localizationand proper function of the enzyme in the liver. We have been particularlyinterested in how the two transcription start sites are controlledin response to physiological stimuli in the rat. To elucidatethe mechanism of the transcriptional regulation responsible forthe alternative subcellular destinations of rat SPT, we recentlyinvestigated the downstream promoter and possible activators includingC/EBP $alpha$ / $beta$ that regulates transcription from the downstream startsite (19, 20). In this paper, we report that Sp1 and AP-2 $beta$ activate the upstream promoter responsible for the generationof rat SPTm-mRNA.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Expression Vectors-- Various fragments of the rat SPT gene were prepared by complete or partial enzyme digestion of cRGspt1 (4), a genomic DNAclone of rat SPT, and inserted into the HindIII or XhoI-NheI siteof pGV-B (Nippongene), a luciferase reporter plasmid without promotersand enhancers. Nucleotide positions of the 5'-ends (the upstreamtranscription start site is numbered +1) of the digested fragmentsinserted into corresponding reporter constructs are as follows: $-$ 5500 (BamHI) for pGBBN550, $-$ 4300 (PstI) for pGBPN430, $-$ 2700 (NcoI)for pGBNN270, $-$ 2400 (PstI) for pGBPN240, $-$ 1256 (HindIII) for pGBHN129, $-$ 386 (NheI) for pGBNN42, $-$ 276 (SmaI) for pGBSN31, $-$ 191 (PvuII)for pGBPN23, $-$ 102 (EcoNI) for pGBENN13, and $-$ 50 (BanIII) for pGBBN9.The 3'-ends of the SPT gene in these constructs are all +36 (NheI).The pTA-Sp1-Luc, pTA-AP-2-Luc, and pTA-Sp1AP-2-Luc plasmids wereprepared by insertion of the $-$ 125 to $-$ 89 region, the $-$ 14 to +10region, and both of these regions of the SPT gene into pTA-Lucplasmid (Clontech Laboratories, Inc.), respectively. Site-directedmutagenesis for construction of reporter plasmids containing mutantSPT promoters, M1 and M2, was performed by PCR-mediated splicingafter overlap extension. In the initial steps, the left arm ofthe PCR product was generated from the wild-type SPT gene encompassingthe $-$ 386 to +36 region using a sense-SPT primer with a HindIIIsite at the 5'-end and an antisense primer containing the desiredmutations. Similarly, the right arm of the PCR product was generatedusing an antisense-SPT primer with an NheI site at the 3'-endand a sense primer containing the mutations. Amplified DNAs weregel-purified and subjected to the second step of PCR using thesense-SPT primer and the antisense-SPT primer. The amplified productswere then digested with HindIII and NheI and were subcloned intothe HindIII-NheI site of pGV-B. Other site-directed alterations(for M3-M9) were made in wild-type pGBNN42 by the LA-PCR method(21) using two complementary oligonucleotides with the desiredmutations, followed by DpnIdigestion.

A wild-type AP-2 $beta$ expression vector, pCMX-AP-2 $beta$ , was kindly donated by Dr. Reinhard Buettner, University Hospital RWTH, Germany(22), and Dr. Hitoshi Okazawa, University of Tokyo, Japan (23),and a wild-type Sp1 expression vector, RSV-Sp1, was a generousgift from Dr. Naoko Tanese, New York University Medical Center.To make another AP-2 $beta$ expression vector, AP-2 $beta$ cDNA within pCMX-AP-2 $beta$ was excised and subcloned into a different expression vector,SP(RSV), which was a kind gift from Dr. Robert Tjian, Universityof California, Berkeley, CA, because the pCMX vector itself severelysuppressed the luciferase expression derived from the reporterconstructs. An expression vector for the N-terminal truncatedAP-2 $beta$ , AP-2 $beta$ $Delta$ N291, was generated by PCR amplification using a5'-primer containing a FLAG sequence followed by subcloning intothe SP(RSV) vector. For preparation of an Sp1 $Delta$ N expression vector,an Sp1 cDNA fragment corresponding to the DNA-binding domain atamino acids 516-696 was amplified by PCR and subcloned into pcDNA3.1-FLAG,which was a generous gift from Dr. Toshiaki Suzuki, Tokyo MetropolitanInstitute of Medical Science, Tokyo, Japan (24). All PCR-mediatedconstructs were subjected to DNA sequencing to verify the clones.Mutant oligonucleotides for the individual sites (mutant basesare in boldface and underlined) are as follows: M1, 5'-GCTATGGAATACTGGGACTCAGGTG-3',with mutation of the inverted repeat (GAACCCCGGGGCTC, locatedat bp $-$ 280 to $-$ 272); M2, 5'-CTTGCTCTCACACACTTGAAAC-3',with mutation of the first AP-1-like site (TGACTCT, located atbp $-$ 218 to $-$ 212); M3, 5'-ACCAGAGGCGTCCCTTCTCCTGTGGAAG-3',with mutation of the Sp1 site (TCCCCTCCCCC, located at bp $-$ 116to $-$ 106); M4, 5'-GGTCAAATTGACTGTAGAAGGGCTGGAG-3',with mutation of the TATA-like site (AATAAAA, located at bp $-$ 31to $-$ 25); M5, 5'-ATAAAAGGGCACGACCAAGCAACAGG-3', withmutation of the C/EBP-like site (TGGAGCAAG, located at bp $-$ 20to $-$ 12); M6, 5'-AAGCAACAGGTACGCACCAACCAG-3', withmutation of the second AP-1-like site (GGACTCA, located at bp $-$ 4 to +2); M7, 5'-AAGCAACAGGGACTTGCCAACCAG-3', with mutationof the transcription start site (CA); M8, 5'-CAACAGGGACTCATTAGCCAGGCCT-3',with mutation of the AP-2 site (TCACCAACCA, located at bp $-$ 1 to+9); and M9 (antisense primer), 5'-CCAGCTAGCTCTGGGCTAAACCTAGCGGCG-3',with mutation of the CRE-like site at bp +21 to +28. Expressionvectors for CBP were described previously (25). A cDNA cloneof E1A was provided by Dr. Marc Montminy, The Salk Institute forBiological Studies, (26), and subcloned into the expressionvector pRC/CMV. Expression vectors for E1A $Delta$ N and E1A $Delta$ CR2 weregenerated by PCR amplification on the basis of information onthe domain structure of E1A reported by Wang et al. (27).

DNase I Footprinting and Gel Mobility Shift Assay-- HepG2 nuclear extracts were prepared as described previously (19). The DNase I footprinting assay was performed accordingto the protocol described by Johnson et al. (28) with some modifications.Briefly, the end-labeled DNA fragment (10-20 fmol) was incubatedon ice for 30 min with the indicated amounts of nuclear extractsin a 50-µl reaction mixture containing 50 mM Hepes-KOH (pH 7.9),1 mM EDTA, 1 mM dithiothreitol, 50 mM KCl, 5% (v/v) glycerol,2.5 µg of bovine serum albumin, and 2 µg of poly(dI-dC). FivemM CaCl₂ and 5 mM MgCl₂ were then added to the reaction mixture,and the mixture was preincubated at room temperature for 5 min,after which 0.07-0.1 units of DNase I was added to digest theDNA at room temperature for 1 min. The reaction was stopped byadding 200 µl of a stop buffer (0.3 M sodium acetate, 25 mM EDTA,25 µg/ml tRNA), and the mixture was then subjected to phenol-chloroformextraction, ethanol precipitation, and electrophoresis on a sequencinggel. In the gel mobility shift assay, a ³²P-labeled double-strand DNA probe (10 fmol) was incubated with4 µg of nuclear extracts under previously described conditions(19). For oligonucleotide competition and supershift experiments,50-200-fold molar excess of annealed oligonucleotides, 1 µg ofantibody against AP-2 $alpha$ , AP-2 $beta$ , AP-2 $gamma$ , or Sp1 (Santa Cruz Biotechnology,Inc., Santa Cruz, CA), or preimmune IgG was preincubated withnuclear extracts on ice for 20 min before addition of a labeledDNA probe. The mixture was then incubated with the probe on icefor another 30 min and applied to a nondenaturing gel (5% polyacrylamide,10% glycerol, 0.25× Tris borate/EDTA buffer), followed by electrophoresisat 10-12.5 mA at 4 °C for 1.5 h. For preparation of probes andcompetitors for gel mobility shift analysis, the following complementaryoligonucleotides were used: $-$ 14/+10 region, 5'-AAGCAACAGGGACTCACCAACCAG-3'; $-$ 125/ $-$ 98 region, 5'-ACCAGAGGCTCCCCTCCCCCTGTGGAAG-3'; initiatorregion of adenovirus major late promoter, 5'-TCGTCCTCACTCTCTTCCCCT-3'.Double-strand oligonucleotides for the binding sites of AP-1,AP-2, YY-1, USF-1, CTF/NF1, Sp1, C/EBP, hepatocyte nuclear factor4, and that for a mutated binding site of Sp1 were purchased fromSanta Cruz Biotechnology,Inc.

Cell Culture and Transfection-- Transfection of DNAs into rat hepatocytes was performed by the electroporation method. Primary rat hepatocytes were preparedby liver perfusion with collagenase as described previously (1).Isolated hepatocyte suspensions were washed twice in ice-coldphosphate-buffered saline( $-$ ) and resuspended at 5 × 10⁶ cells/ml in ice-cold phosphate-buffered saline( $-$ ). Then 0.8 mlof the suspension was mixed with equal moles of a reporter construct(15-25 µg, total amount of DNA being equalized to 25 µg by theaddition of the pGV-B plasmid), 10 µg of RSV- $beta$ -galactosidase (anexpression vector for $beta$ -galactosidase), and 50 µg of salmon testisDNA in a Gene Pulser cuvette with a 0.4-cm electrode (Bio-Rad)and incubated on ice for 15 min. After resuspending the mixturegently, hepatocytes were exposed to a pulse at 280 V/960 microfaradsand incubated on ice for 10-15 min for recovery. Cells were thentransferred carefully into 7.2 ml of an ice-cold maintenance medium(Williams E medium with 10% fetal bovine serum, 25 µg/ml kanamycin,25 µg/ml Cefamezin, 1 nM insulin, and 25 µg/ml epidermal growthfactor), suspended very gently, seeded into 4 wells of a 6-welldish, and incubated in 5% CO₂, 30% O₂ at 37 °C for 6 h. The mediumwas then changed to a fresh maintenance medium with (8-Br-cAMP)or without (control) 0.1 mM 8-Br-cAMP, and the culture was continuedfor another 24 h, followed by measurement of the luciferaseactivity.

For transfection into HepG2 cells, cells grown in Dulbecco's modified Eagle's medium with 10% fetal bovine serum were seededat 5 × 10⁵ cells/well in a 6-well dish, cultured overnight, and transfectedwith plasmids by the calcium phosphate method (29) or with FuGENE6Transfection Reagent (Roche Molecular Diagnostics). The RSV- $beta$ -galactosidaseplasmid (0.05 µg) and an expression plasmid (0.2 µg) for a catalyticsubunit of wild-type PKA $alpha$ (wt-PKA) or a mutant catalytic subunitof PKA $alpha$ (control) were included in the transfection medium inall experiments with HepG2 cells. Where indicated, other plasmidswere also used. Total amounts of plasmids were equalized by addingthe pGV-B plasmid or backbone vector plasmids. Cells were culturedfor another 24 h after transfection and then harvested for measurementof luciferaseactivity.

The luciferase activity in the cell extracts was measured using Pikka gene assay reagent (NIPPON GENE Co., Ltd., Japan) orluciferase assay system (Promega Biosciences, Inc.) and normalizedwith $beta$ -galactosidase activity. The relative luciferase activityrepresents the relative fold value versus that of pGV-B (Fig.1) or versus that of pGBNN42 (Figs. 2, 4, 6, and 7) when transfectedwith the mutant PKA vector. The mutant PKA vector expresses thecatalytic subunit of PKA $alpha$ lacking ATP binding ability but doesnot act in a dominant negative manner. All transfections wereperformed in duplicate and repeated at least threetimes.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Determination of the Proximal Promoter Region for Upstream Transcription Initiation in the Rat SPT Gene-- To identify the region that controls the upstream promoter activity, we performed reporter gene assays using various deletionmutants of the rat SPT gene fused to the luciferase gene. Theseconstructs carry only the upstream transcription start site (+1)as illustrated in Fig. 1A. In our preliminary experiments withprimary rat hepatocytes, low transfection efficiency and weakpromoter activity of the SPT gene made it difficult to obtainreproducible data. Therefore, we tested transfections into threecell lines, human hepatoma HepG2 and rat hepatoma H4IIE and FAA3T3cells, to select cells in which the SPT promoter activity canbe detected more efficiently with a similar pattern to that inprimary rat hepatocytes. In HepG2 cells, all of the 5'-deletionconstructs from $-$ 5500 ~ +36 to $-$ 1256 ~ +36 (Fig. 1A) showed higherbasal and cAMP/PKA-induced promoter activities with a similarpattern to that in primary hepatocytes (Fig. 1B). In the othertwo cell lines, however, transcription efficiencies were as lowas that in primary hepatocytes (data not shown). Based on theseobservations, we decided to use HepG2 cells in all of the followingexperiments.

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Fig. 1. Expression of 5'-deletion mutants of rat SPT-LUC fusion genes in HepG2 cells and primary rat hepatocytes. A, schematic representation of 5'-deletion mutants of the rat SPT gene. Various lengths of SPT 5'-franking regions extending to +36 were fused to the luciferase (LUC) reporter gene. Two predetermined transcription start sites, +1 and +66, are shown by hook-shaped arrows. B, SPT promoter activities in HepG2 and primary rat hepatocytes. An equal mole of each reporter plasmid shown in A was transiently transfected into HepG2 cells (left) with 0.02 µg of a mutant PKA (control) or a wild-type PKA (wt PKA) expression plasmid by the calcium phosphate method, or into primary rat hepatocytes (right) by the electroporation method. For HepG2 cells, the medium was changed 6 h after the transfection with a fresh Dulbecco's modified Eagle's medium containing 10% fetal bovine serum, and the culture was continued for another 24 h. For primary rat hepatocytes, the medium was changed 4 h after electroporation to a serum-free Williams E medium, and cells were incubated in the absence (control) or presence of 0.1 mM 8-Br-cAMP for another 24 h. The luciferase activity was measured as described under "Materials and Methods." Relative LUC activity represents the relative fold value versus the control activity of promoter-less pGV-B plasmid.

Because the region from $-$ 1256 to +36 (pGBNN42 plasmid) maintained a significant PKA responsiveness with 10-12-fold induction,we examined the effect of further deletion to determine the proximalregion involved in the upstream promoter activity of the SPT gene(Fig. 2). Deletions to position $-$ 387 slightly increased the PKA-inducedpromoter activity, suggesting the presence of a weak inhibitoryelement. Deletions to $-$ 277 resulted in about a 30% decrease inthe activity, but the $-$ 191 to +36 region (pGBPN23) maintainedalmost the same level of activity as that of the $-$ 276 to +36 region.Further deletions up to $-$ 103 caused 1/3-1/4-fold reductions. On theother hand, the basal promoter activity was almost unchanged untilthe 5'-end of the gene was shortened to $-$ 50; i.e. the $-$ 50 to +36region (pGBBN9) showed only a very low activity in both controland PKA-transfected cells. Similar results were obtained whencells were stimulated with 0.5 mM 8-bromo-cAMP instead of theintroduction of PKA (data not shown). These data indicate thatthe $-$ 191 to $-$ 51 region contains elements that play important rolesin the upstream promoter activity of the SPT gene.

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Fig. 2. Determination of the proximal promoter region of the upstream promoter. Sequential deletion fragments of the rat SPT gene (solid bar) were fused to the luciferase gene, and an equal mole of the construct was transiently transfected with 0.02 µg of a mutant PKA (control) or a wild-type PKA (wt PKA) expression plasmid. The luciferase (LUC) activity was measured as described under "Materials and Methods." Relative LUC activity represents the relative fold value versus the control activity of pGBNN42 ( $-$ ).

AP-2 $beta$ Binds to the Region Overlapping the Transcription Start Site and Activates the Basal Promoter Activity-- To characterize cis-elements regulating the SPT promoter activity, we performed DNase I footprinting analysis using HepG2nuclear extracts and various SPT gene fragments, including the $-$ 386 to $-$ 277 region and the $-$ 191 to +36 region, as probes. Threemain protected regions were detected, two of which (I and II,Fig. 3A) were located close to or over the transcription startsite, and the other was at $-$ 125 to $-$ 89 (cf. Fig. 5A). No protectedregion was observed within the $-$ 386 to $-$ 277 region (data not shown),although deletion of this region caused a small but obvious reductionin the luciferase activity as shown in Fig. 2.

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Fig. 3. Identification of the AP-2-binding site in the $-$ 14 to +10 region. A, DNase I footprint analysis (left) and gel mobility shift assay (right) with HepG2 nuclear extracts. Radiolabeled fragment of the rat SPT gene at $-$ 191 to +36 was preincubated with various amounts (0-16 µg) of nuclear extract prior to the DNase I digestion. The regions protected by protein binding are indicated with two boxes (I and II). The vertical bar designates the position of the probe used for the gel mobility shift assay. Nucleotide numbers are shown on the left side of the G+A lane, the sequence ladder by G and A digestion. In the right panel, the arrow marks specific protein binding to the $-$ 14 to +10 region ( $-$ 14/+10). The protein-DNA complex was subjected to competition with 50- (lanes 3 and 5) or 200- (lanes 4 and 6-10) fold molar excess of various binding site competitors as indicated at the top. No nuclear extracts were added in lane 1. B, comparison of the protein-DNA complex with the $-$ 14/+10 probe (left) with that formed with a known AP-2-binding site (right). Experimental details are described under "Materials and Methods." Binding site competitors, anti-AP-2 antibodies, and preimmune IgG (PI-IgG) (1 µg each) are indicated at the top. 50× and 100× indicate 50- and 100-fold molar excesses, respectively. C, sequence of the putative AP-2-binding site in the SPT gene in comparison with the consensus AP-2 site. Identical nucleotides are shown by squared dots.

To determine the transcription factors that bind to the I-II region overlapping the transcription start site, we next performedgel mobility shift assays. Because several probes containing eitherregion I or II failed to form any complex with HepG2 nuclear proteins,a DNA fragment of the $-$ 14 to +10 region was also tested as a probe,and eventually this region was found to form a specific protein-DNAcomplex that was detected as a single band (Fig. 3A, right, lane2). As the $-$ 14 to +10 region contained putative binding sitesfor AP-1 and AP-2 (cf. Fig. 7A), we then used those consensussites as competitors. Effective competition for the protein-DNAbinding was observed by addition of a 50-fold molar excess ofan unlabeled self-fragment and the consensus AP-2 site, whereasthe consensus AP-1 site only slightly weakened the signal of theband (Fig. 3A, right, lanes 3-5). Other competitors, includingthe adenovirus major late initiator and the consensus bindingsites for C/EBP, Sp1, and initiator-binding factors such as YY-1,USF-1, and CTF/NF1, did not show any effects on the complex formation.Indeed, the DNA sequence of 5'-TCACCAACCA-3' at position $-$ 1 to+9 in the SPT gene had a high homology with the consensus AP-2site (Fig. 3C) found in the human metallothionein II_A gene (29).As shown in Fig. 3B, preincubation of nuclear extracts with ananti-AP-2 $beta$ antibody prevented the formation of protein-DNA complexes,suggesting that AP-2 $beta$ is capable of binding to the sequence. Anantibody against AP-2 $alpha$ also inhibited the complex formation butthe effect was more partial. On the other hand, inhibition byan anti-AP-2 $gamma$ antibody was not significant under the experimentalconditions used. An antibody against c-Fos had no effect (datanot shown). Similar results were obtained when the consensus AP-2site was used as a probe (Fig. 3B, right). These results suggestthat AP-2 $beta$ binds to the $-$ 14 to +10 region of the SPT gene in vitro.

We next investigated the possible function involvement of AP-2 $beta$ in the regulation of SPT gene expression. For this purpose,AP-2 $beta$ was overexpressed in a transient reporter assay using pGBNN42(Fig. 4). Expression of wild-type AP-2 $beta$ caused a 6-8-fold inductionof basal promoter activity of the SPT gene in a dose-dependentmanner. PKA-induced activity was also enhanced by wild-type AP-2 $beta$ but, unexpectedly, only to about the same level as that of theAP-2 $beta$ -induced basal activity or even to a lower level, dependingon the amount of AP-2 $beta$ transfected. No cAMP/PKA-induced increasein the level of AP-2 $beta$ was detected under the experimental conditionsused (data not shown). Therefore, the above results suggest thatAP-2 $beta$ can activate basal transcription without being involvedin the PKA-induced expression of mitochondrial SPT. Western blotanalysis showed that the AP-2 $beta$ level in PKA- or cAMP-stimulatedHepG2 cells transfected with a large amount of an AP-2 $beta$ expressionplasmid was slightly lower than that in nonstimulated cells transfectedwith the same amount of the plasmid (data not shown). This maybe a reason why the PKA-induced activity was lower than the basalactivity when a higher amount of AP-2 $beta$ was expressed (Fig. 4,center column). Ectopic expression of AP-2 $alpha$ also enhanced thebasal promoter activity (data not shown), suggesting that thereis no subtype specificity within AP-2 transcription factors. AP-2has been shown to bind to DNA as a dimer, with the binding anddimerization domains located within the C-terminal half of theprotein (31). An N-terminal-truncated AP-2 $alpha$ region, $Delta$ N278, containingonly the dimerization domain is unable to bind to DNA but retainsthe ability to dimerize with the wild-type protein, thereby preventingbinding of the latter to DNA (32). As the dimerization domainwas highly conserved among the AP-2 subtypes, we expected thatthe homologous domain of AP-2 $beta$ (amino acids 292 to the C-terminalend) might serve as a dominant negative factor. Indeed, coexpressionof AP-2 $beta$ $Delta$ N291 inhibited the AP-2 $beta$ -induced promoter activity regardlessof whether the cells had been co-transfected with PKA or not (Fig.4). Single transfection of the AP-2 $beta$ $Delta$ N291 expression plasmid withoutwild-type AP-2 $beta$ caused only a slight reduction in the basal promoteractivity (data not shown), probably because the endogenous AP-2level in HepG2 cells was very low (30, 33). Based on thesedata, we conclude that AP-2 $beta$ has the ability to elevate SPT expressionby interaction with the region overlapping the transcription startsite and that the function of AP-2 is independent of PKA activation.

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Fig. 4. Enhancement by AP-2 $beta$ of basal activity of the upstream promoter. One µg of pGBNN42 was transiently transfected into HepG2 cells with a mutant (control) or wild-type (wt PKA) PKA expression plasmid in the presence or absence of wild-type AP-2 $beta$ expression plasmid (0.02 µg, +, or 0.06 µg, ++) or AP-2 $beta$ $Delta$ N291 expression plasmid (0.06 µg, +, or 0.125 µg, ++). The luciferase activity was measured as described under "Materials and Methods." Relative LUC activity represents the relative fold value versus the control activity of pGBNN42 ( $-$ ).

Sp1 Is Involved in Both Basal and PKA-induced Promoter Activities-- Another possible region responsible for regulation of the upstream promoter activity as determined by DNase I footprint analysiswas the region covering positions $-$ 125 to $-$ 89, as shown in Fig.5A (left panel). Fig. 5C shows a C-rich motif in this region thatis homologous to the consensus Sp1 site (34, 35). In the gelmobility shift assay, specific protein binding to the $-$ 125 to $-$ 89 region (Fig. 5, A, right, lanes 2 and 7) was diminished bya 50-fold molar excess of a self-competitor and a DNA fragmentcontaining the Sp1 site (Fig. 5A, right, lanes 3, 4, and 8) butnot by binding sites for C/EBP, AP-1, hepatocyte nuclear factor4, and AP-2 (Fig. 5A, right, lanes 5, 6, 9, and 10) or a DNA fragmentof a mutant Sp1 site (Fig. 5B, lane 5). The DNA-protein complexwas supershifted by the addition of an anti-Sp1 antibody (Fig.5B, lane 6). Similarly, the consensus Sp1 site used as a probealso formed a specific complex with HepG2 nuclear extracts, andthe complex was supershifted by the addition of an anti-Sp1 antibody(Fig. 5B, right). All these data indicate that the $-$ 125 to $-$ 89region contains an Sp1-binding site.

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Fig. 5. Identification of the Sp1-binding site in the $-$ 125 to $-$ 89 region. A, DNase I footprint analysis (left). A radiolabeled fragment ( $-$ 191 to +36) of the rat SPT gene was preincubated with various amounts (0-40 µg) of HepG2 nuclear extracts prior to DNase I digestion. The regions protected by protein binding are indicated by a box and the vertical sequences with nucleotide numbers. Right, gel mobility shift assay using the $-$ 125 to $-$ 89 region ( $-$ 125/ $-$ 89) as a probe. The assay was performed in the absence (lanes 1, 2, and 7) or presence of 50-fold (lanes 3, 4, and 8) or 200-fold (lanes 5, 6, 9, and 10) molar excesses of binding site competitors as indicated at the top. No nuclear extracts were added in lane 1. An arrowhead shows a specific protein-DNA complex. B, comparison of protein-DNA complex with the $-$ 125/ $-$ 89 probe (left) with that formed with a known Sp1-binding site (right). Binding site competitors (50-fold molar excess), anti-Sp1 antibody (1 µg), and preimmune IgG (PI-IgG) (1 µg) are indicated at the top. Asterisks indicate nonspecific bands. C, comparison of the putative Sp1-binding site in the SPT gene with the consensus Sp1 site. Identical nucleotides are shown by squared dots.

Functional involvement of Sp1 in the regulation of SPT gene transcription was then demonstrated by the results of a transientreporter gene assay (Fig. 6A). Enforced expression of wild-typeSp1 enhanced basal promoter activity of SPT to produce markedelevation of PKA-induced activity in a dose-dependent manner,whereas a truncated Sp1 lacking the N- terminal activation domainand possessing only the DNA-binding domain (36) prevented thepromoter activation as a dominant negative factor. The -fold inductionby PKA relative to basal activity was almost unchanged, althougha slight increase was observed in some experiments. These resultssuggest that Sp1 is involved in both basal and PKA-induced expressionof the SPT gene mainly by activating the basal promoter.

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Fig. 6. Involvement of Sp1 in basal and PKA-induced activities of the upstream promoter. A, effects of wild-type Sp1 and a mutant Sp1 (Sp1 $Delta$ N). One µg of pGBNN42 was transiently transfected into HepG2 cells with a mutant (control) or wild-type PKA expression plasmid in the presence or absence of an expression plasmid for wild-type Sp1 (0.125 µg, +, or 0.25 µg, ++) or mutant Sp1 (Sp1 $Delta$ N, 0.125 µg, +, or 0.25 µg, ++). The luciferase (LUC) activity was measured as described under "Materials and Methods." Relative LUC activity represents the relative -fold value versus the control activity of pGBNN42 ( $-$ ). B, effect of coexpression of CBP on the enhancement by Sp1. The reporter gene assay was performed as described in A, except that an expression plasmid for wild-type Sp1 (0.25 µg) was transfected in combination with a CBP plasmid (0.1 µg, +, or 0.3 µg, ++). C, inhibition by adenovirus E1A of the upstream promoter activity. pGBNN42 was transfected into HepG2 cells with a mutant (control) or wild-type PKA expression plasmid as in A, except that 0.003 µg of an expression plasmid for wild-type E1A or mutant E1A (E1A $Delta$ N and E1A $Delta$ CR2) was also transfected. D, reversal by CBP of E1A-mediated inhibition of SPT promoter activity. The reporter gene assay was performed as described in C, except that an expression plasmid for wild-type E1A was transfected in combination with a CBP plasmid (0.05 µg, +, 0.1 µg, ++, or 0.3 µg, +++).

CBP Augments the PKA-induced and Sp1-enhanced SPT Promoter Activity as a Coactivator-- Recently, Sp1 has been shown to be associated with CBP, a general coactivator for a number of transcription factors, to displayits regulation of the target gene expression (37, 38). Indeed,introduction of CBP enhanced PKA-induced promoter activity ofSPT (Fig. 6B). Besides, coexpression of CBP with Sp1 was moreeffective in the enhancement than expression of CBP or Sp1 alone.On the other hand, CBP did not affect AP-2 $beta$ -induced promoter activityat all (Fig. 7C), consistent with the fact that no direct interactionbetween AP-2 $beta$ and CBP has been reported at present. Ectopic expressionof wild-type E1A severely repressed the PKA-induced promoter activity(Fig. 6C), and CBP overcame the repression by E1A (Fig. 6D). Thisresult indicated the participation of CBP, because E1A has beenshown to inhibit CBP-dependent transcription because of its highaffinity for CBP, thus preventing CBP-RNA polymerase II interaction(26, 39). Inhibition was also observed when a mutant E1A lackingthe Rb-binding domain (E1A $Delta$ CR2) was co-transfected. However, amutant E1A lacking the CBP-binding domain (E1A $Delta$ N) failed to repressthe activity, suggesting specific participation of CBP. Becauseit has recently been shown that Sp1 function is activated by PKA,these findings suggest that the enhancement by PKA of the upstreampromoter is mediated by activation of Sp1, which functions throughassociation with CBP. On the other hand, Sp1-enhanced basal promoteractivity was not affected by CBP (Fig. 6B), and its inhibitionby wild-type E1A was minimal, if any (Fig. 6C). These resultssuggest that Sp1 elevates the basal promoter activity througha different mechanism. The reason for the small increase in basalpromoter activity caused by E1A $Delta$ N and E1A $Delta$ CR2, observed in theresults shown in Fig. 6C, is unknown.

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Fig. 7. Involvement of the binding sites for AP-2 and Sp1 in the upstream promoter activity. A, effects of various mutations in the $-$ 386 to +36 region on promoter activity. Schematic diagram (bottom) represents putative cis-elements found in the $-$ 386 to +36 region and various mutants of the pGBNN42 plasmid. Wild-type (WT) or a mutant (M1-M9) pGBNN42 plasmid (1.5 µg each) was transfected into HepG2 cells, and the reporter gene assay was performed as described under "Materials and Methods." Relative LUC activity represents the relative -fold value versus the control activity of wild-type pGBNN42 ( $-$ ). B, effects of mutations within the putative Sp1 or AP-2 site on protein-DNA binding. Gel mobility shift assays were performed with HepG2 nuclear extracts and the $-$ 125 to $-$ 89 region ( $-$ 125/ $-$ 89) or the $-$ 14 to +10 ( $-$ 14/+10) region of the SPT gene as a probe. For the competition assay (lanes 3, 4, and 7-9), the nuclear extracts were preincubated with a 50-fold molar excess of unlabeled annealed oligonucleotides of the wild-type sequence ( $-$ 125/ $-$ 89wt, $-$ 14/+10wt) or mutant sequences having mutations shown in A ( $-$ 125/ $-$ 89m3, $-$ 14/+10m7, and $-$ 14/+10m8) prior to the addition of the probe. C, functional involvement of Sp1 in the promoter activity through binding to the $-$ 125 to $-$ 89 region. One µg of wild-type or mutant (M3) pGBNN42 was transiently transfected with an expression plasmid for Sp1 (0.25 µg), AP-2 $beta$ (0.125 µg), CBP (0.3 µg), or CBP in combination with the Sp1 or AP-2 $beta$ plasmids. The reporter gene assay was performed as described under "Materials and Methods." Relative LUC activities represent the relative fold value versus the control activity of wild-type pGBNN42 ( $-$ ).

The Sp1 Site and AP-2 Site Are Functional cis-Elements within the Upstream Promoter-- To confirm that Sp1 and AP-2 serve as trans-activators of the SPT upstream promoter through their binding to specific DNAelements, we carried out transient reporter assays and gel mobilityshift assays using a series of mutant pGBNN42 constructs and mutantSPT gene fragments (Fig. 7). As shown in Fig. 7A, introductionof mutations into the putative Sp1 site (M3) caused a 1/3-fold decreasein the PKA-induced promoter activity. However, this reporter constructdid not alter the basal promoter activity, despite the observationthat the basal activity was enhanced by overexpression of Sp1(cf. Fig. 6B). Although the reason for this is not clear, onepossibility is that the Sp1 action through the $-$ 125 to $-$ 89 regioncontributes largely to the PKA-induced activity rather than tothe basal activity and another unidentified Sp1 site locates withinthis promoter region. The Sp1 binding to the $-$ 125 to $-$ 89 regionwas not abrogated by an unlabeled DNA fragment containing a mutantSp1 site ( $-$ 125/ $-$ 89m3, Fig. 7B, left). In addition, enforced expressionof Sp1 caused only a slight increase in the promoter activityof the SPT gene containing the mutant Sp1 site (M3, Fig. 7C).On this mutant promoter, CBP could not exert its coactivator functionirrespective of Sp1 expression. These results indicate that the $-$ 125 to $-$ 89 region is necessary for both the binding of and thepositive regulation of the PKA-induced promoter activity bySp1.

Mutations within the putative AP-2 site resulted in a substantial decrease in both basal and PKA-induced promoter activitiesof the SPT gene (M7 and M8, Fig. 7A). In the case of M7, whichhas mutations at positions +1 and +2 in the SPT gene, the repressionof the promoter activity seems to be due to inhibition of theformation of basal transcriptional machinery, because AP-2 bindingto the $-$ 14 to +10 region was inhibited by an oligonucleotide ( $-$ 14/+10m7)carrying the same mutation as that of M7 as strongly as that bythe wild-type self-competitor ( $-$ 14/+10wt) (Fig. 7B). In the caseof M8, it is likely that the decrease is caused by inhibitionof the binding of AP-2 $beta$ to DNA, considering that mutated oligonucleotide, $-$ 14/+10m8, was unable to compete for the binding (Fig. 7B, lane8). Because the AP-2-binding site overlaps the transcription startsite, AP-2 and its target element may contribute to the initiatorcomplex so that mutations in this site might cause severe damageto the promoter context. That might be a reason why both basaland PKA-responsive activities were greatly reduced. In supportof our tentative conclusion that AP-2 $beta$ acts without having anycorrelation with the Sp1 binding to the $-$ 125 to $-$ 89 region, enforcedexpression of AP-2 $beta$ elevated the basal activity of the M3 constructto the same degree as that achieved with the wild-type construct(Fig. 7C).

Mutations within other regions in the SPT gene had no effect. CRE-, AP-1-, and TATA-like sites are not significantly involvedin the upstream promoter activity of SPT in this reporter assaysystem. Indeed, overexpression of CREB, AP-1, and TBP (TATA-boxbinding protein) was not effective on the promoter activation(data not shown). Also, the C/EBP-like site ( $-$ 20 to $-$ 12) doesnot seem to regulate SPTm expression although C/EBP $alpha$ / $beta$ bindsto the region overlapping the downstream start site to mediatethe production of SPTp-mRNA (20).

The finding that AP-2 and Sp1 serve as positive regulators in the activation of the SPT promoter through their binding tothe respective specific cis-elements prompted us to ask whetherSp1 and AP-2 can also function as cAMP/PKA-responsive factorsfor a neutral promoter. We next constructed luciferase plasmidsin which the Sp1 and/or AP-2 site of the SPT gene was fused withthe minimal promoter of the herpes simplex virus-thymidine kinasegene containing the TATA-box but not other regulatory elements(the resulting plasmids were denoted pTA-Sp1-Luc, pTA-AP-2-Luc,and pTA-Sp1AP-2-Luc), and transfected these constructs into HepG2cells. Introduction of the Sp1 or AP-2 site resulted in 2-3-foldinduction of the basal activity of the minimal promoter. Also,introduction of both of these sites enhanced the basal activityby 16-17-fold (Fig. 8). However, unlike the results obtained withluciferase plasmids containing the SPT promoter, stimulation by8-bromo-cAMP did not affect the luciferase activities when neitherSp1 nor AP-2 plasmid was cotransfected. Overexpression of Sp1or AP-2 $beta$ elevated the basal activity a further 1.5-2-fold, andSp1 caused moderate cAMP responsiveness only with the pTA-Sp1-Lucplasmid. Thus, the Sp1 and AP-2 sites of the SPT gene introducedupstream of the TATA-box within the herpes simplex virus-thymidinekinase minimal promoter do not function as cAMP-responsive elementseffectively, although these sites play roles in the enhancementof the basal activity of the minimal promoter. These results indicatethat the core promoter context of the SPT gene is important forits full cAMP responsiveness or that other unidentified cis-element(s)might be required.

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Fig. 8. Effect of Sp1- and AP-2-binding sites on thymidine kinase minimal promoter. Sp1- and/or AP-2-binding sites of the SPT gene were fused to the minimal promoter of the herpes simplex virus-thymidine kinase gene within a pTA-Luc plasmid. Each luciferase plasmid (0.5 µg) was transiently transfected with an expression plasmid for Sp1 (0.25 µg) or AP-2 $beta$ (0.125 µg). Cells were incubated in the presence of 0.1 mM 8-Br-cAMP for the last 24 h of the transfection. Relative LUC activities represent the relative fold value versus the control activity of pTA-Luc ( $-$ ).

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In this study, we demonstrated the roles of specific cis-acting sequences and transcription factors in the regulation of theupstream promoter activity for generation of rat SPTm-mRNA. Weidentified two transcription factors, AP-2 $beta$ and Sp1, which areinvolved only in activation of basal promoter and in both basaland PKA-induced promoter activity,respectively.

Some notable features of AP-2 $beta$ should be noted before considering its role in regulation of SPT gene expression. First, AP-2 $beta$ enhanced only the basal promoter activity and no further activationwas observed upon expression of a catalytic subunit of PKA. Second,the binding site of AP-2 $beta$ is in a region overlapping the upstreamtranscription start site. It has been shown that AP-2 transcriptionfactors play important roles in the regulation of gene expressionresponsible for vertebrate embryonic development, differentiationof epidermal cell lineages (40, 41), tumorigenicity of variouscancer cells (42), and cell cycle control (43). To respondto various signals for the regulation of the above mentioned cellfunctions, the AP-2 activity is modulated through different signaltransduction pathways. Phorbor ester along with cyclic AMP inducesAP-2 activity to enhance transcription of the human metallothioneinIIA gene without de novo protein synthesis (30). Park et al.(44) showed that AP-2 was phosphorylated by protein kinase Ato mediate insulin induction of the acetyl-CoA carboxylase geneexpression. It is also reported that retinoic acid induces AP-2activity by increasing AP-2 mRNA levels in human teratocarcinomacells (45). Based on the above information, we first expectedthat AP-2 might mediate the PKA responsiveness of the upstreampromoter activity of the SPT gene. However, only the basal promoteractivity was enhanced by overexpression of AP-2 $beta$ . AP-2 $beta$ may serveas an initiator-like factor, such as YY-1, USF1, or TFII-I, infunctional association with other general transcription factors,but independent of the cAMP/PKA-signalingpathway.

Another point to be discussed is AP-2 in hepatic cells. Although our data clearly showed positive regulation by AP-2 $beta$ of SPTgene expression, AP-2 is known to be primarily expressed in neuralcrest cells and related cells but not significantly in endodermallyderived tissues such as the liver or in hepatoma cells, includingHepG2 cells. This may provide at least a partial explanation forthe low basal level of SPTm-mRNA in vivo (1).

Both basal and PKA-induced activities of the upstream promoter were elevated by overexpression of Sp1, suggesting that Sp1is one of the mediators of the cAMP/PKA signaling pathway in SPTexpression. Sp1 was originally identified as a specific factorrequired for simian virus 40 transcription (46) and has beencharacterized as a ubiquitous transcription factor that servesto maintain the basal level of transcriptions for constitutiveexpression of many other genes, including the adenosine deaminasegene (47), herpes simplex virus-thymidine kinase gene (48),epidermal growth factor receptor gene (49), and DNA polymerase $beta$ gene (50). Interaction of Sp1 with TBP (51), TAFII130 (52),and RNA polymerase II (53) has been demonstrated to be involvedin the regulation of basal transcription by Sp1. The activationfunction of Sp1 has been mapped to its N terminus, which containsglutamine- and serine/threonine-rich domains (36). AlthoughSp1 is a constitutive transcription factor, several research groupshave recently reported that Sp1 function might also be importantin tissue-specific and developmental regulation of gene expression(54). For this regulation, Sp1 has often been shown to meditatecAMP-induced activation of gene expression. For example, Sp1 hasbeen shown to confer cAMP responsiveness on the bovine CYP11Apromoter (55). Rohlff et al. (56) showed that modulation ofSp1 by PKA causes an increase in the DNA binding activity andtrans-activating properties of Sp1. Thus, it is likely that Sp1has the ability to regulate the PKA-induced activation of SPTgeneexpression.

As in the case of many transcription activators/enhancers, Sp1 has been shown to be associated with CBP in response to hormonalstimuli via activation of other transcription factors (36, 37).It has been demonstrated that CBP recruits RNA polymerase II onthe transcription start site of target genes by bridging interactionbetween activator/enhancer and RNA polymerase II (25, 26)and that adenovirus E1A prevents the interaction by competitivebinding to CBP through its N- terminal CBP-binding domain (27,39, 57). Our data in this study support these reports andsuggest that Sp1 is one of the major regulators of the upstreampromoter activity for the generation of SPTm-mRNA.

The mechanism by which Sp1 mediates cAMP-induced expression of SPT is still unclear. Hormonal regulation of Sp1 expressioncould be one of the possible mechanisms. Alternatively, DNA bindingactivity may be modulated by phosphorylation by PKA (56). However,the expression level of Sp1 in HepG2 cells determined by Westernblotting was hardly affected by 8-Br-cAMP. In addition, if thecAMP/PKA-induced expression of SPT were mediated merely by Sp1expression, PKA would not cause further enhancement of SPT inthe presence of sufficient Sp1, but this was not the case. Furthermore,the signal of DNA-protein complex in the gel shift assay was notincreased when nuclear extracts from cAMP-stimulated or PKA-overexpressedHepG2 cells were used (data not shown), suggesting that neitherthe expression nor the DNA binding activity of Sp1 was increasedby cAMP/PKA. Another possible explanation is that PKA regulatesinteractions of Sp1 with other factors. Sp1 can interact withseveral other transcription factors (58, 59), and it enhancescooperative interactions to link their trans-activation domainsto the transcription initiation complex (60, 61). Furtherstudies along this line are needed to fully understand how Sp1functions in the regulation of the SPTpromoter.

The results of the reporter analysis revealed distinct activity of the binding regions for Sp1 and AP-2 in the SPT gene whenthese regions were introduced upstream of a minimal promoter ofthe herpes simplex virus-thymidine kinase gene, suggesting thatspecific promoter context and cross-talk of other transcriptionfactors through additional regulatory regions may be necessaryfor Sp1- and AP-2-mediated promoter activation of the SPT gene.We had expected to find positive involvement of CREB, AP-1, andTBP, because there is one CRE-like element, two AP-1-like elements,and one TATA-like element within the $-$ 386 to +36 region of theSPT gene (Fig. 7). CREB and/or AP-1 have been shown to be mediatorsof cAMP/PKA-dependent transcription (62, 63). The TATA-likeelement (AATAAAA) is located about 30 bp upstream of the startsite (+1) within the SPT gene, and a minor mutation (the firstT to A) has been reported to give little effects on a TATA-dependentpromoter activity (64). In this study, however, we found thatthese putative elements did not act for the SPT promoter. Thus,the rat SPT gene may possess a unique promoter from which SPTm-mRNAsynthesis is TATA-independent despite the existence of this sequenceand no canonical initiator factor contributes to its regulation.Further investigation will be necessary to rule out the possibilitythat the truncated promoter fused to a heterologous reporter geneis regulated differently from the endogenous SPTpromoter.

As described in the Introduction, SPT has the unique feature that its transcriptional regulation is closely liked to its specificorganelle localization depending on the feeding habits of theanimal species. In the rat SPT gene, the downstream transcriptionstart site is used for maintaining a steady level of SPT in peroxisomesto metabolize hepatic glyoxylate, whereas transcription from theupstream site is greatly activated in response to an increaseof intracellular cAMP to produce mitochondrial SPT when a highprotein diet causes a robust release of glucagon. Generation ofSPTp-mRNA from the downstream transcription start site is dominantin a steady state condition and does not significantly respondto cAMP/PKA signaling. We have recently reported that C/EBP $alpha$ / $beta$ binds to the region overlapping the downstream transcription startsite to activate the transcription of SPTp-mRNA (20). However,the C/EBP-like site within the upstream promoter region did notcontribute to transcription from the upstream start site. In lightof these facts, we think it likely that C/EBP plays a dominantrole as a key factor for liver-specific transcription in regulatingthe downstream promoter, so that regulatory elements for the upstreampromoter cannot function. Conformational change of the promoterarchitecture by cAMP/PKA-signaling might switch the upstream siteto a major transcription start site under control by the Sp1-CBPinteraction. It would be interesting to determine whether Sp1activates or inactivates the transcription from the downstreamsite. In our previous study, Northern blot analysis and a nuclearrun-on assay with primary rat hepatocytes indicated that inductionof SPTm-mRNA via a cAMP/PKA signaling pathway required on-goingprotein synthesis (1). Because the expression levels of Sp1and AP-2 $beta$ did not significantly increase in HepG2 cells stimulatedwith 8-Br-cAMP, unidentified factor(s) may also be involved inPKA-induced generation of SPTm-mRNA in vivo. Further studies willfocus on molecular details of how the different transcriptioninitiations from the two separate sites are regulated for properarrangement of the gene products incells.

ACKNOWLEDGEMENTS

We thank Drs. Hitoshi Okazawa and Reinhard Buettner for kindly providing the AP-2 $beta$ expression vector. We are grateful to Dr.Naoko Tanese for providing the Sp1 expression vector and Dr. RobertTjian for providing SP(RSV) plasmid. We are also grateful to Dr.Toshihiro Nakajima, St. Marianna University School of Medicine,for helpful suggestions during the course of thisstudy.

	FOOTNOTES

^* This work was supported by grants-in-aid from the Ministry of Education, Culture, Sports, Science and Technology of Japan(to C. U. and M. K.).The costs of publication of this articlewere defrayed in part by the payment of page charges. The articlemust therefore be hereby marked "advertisement" in accordancewith 18 U.S.C. Section 1734 solely to indicate thisfact.

^§ To whom correspondence should be addressed. Tel.: 81-53-435-2324; Fax: 81-53-435-2323; E-mail: cuchida@hama-med.ac.jp.

Published, JBC Papers in Press, August 6, 2002, DOI 10.1074/jbc.M201380200

ABBREVIATIONS

The abbreviations used are: SPT, serine:pyruvate aminotransferase; AP-1, activator protein 1; AP-2, activator protein 2; CBP, CREB-binding protein; C/EBP, CCAAT/enhancer-binding protein; CREB, cAMP-responsive element-binding protein; PKA, protein kinase A; RSV, Rous sarcoma virus; 8-Br-cAMP, 8-bromo-cAMP.

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The Role of Sp1 and AP-2 in Basal and Protein Kinase A-induced Expression of Mitochondrial Serine:Pyruvate Aminotransferase in Hepatocytes*

The Role of Sp1 and AP-2 in Basal and Protein Kinase A-induced Expression of Mitochondrial Serine:Pyruvate Aminotransferase in Hepatocytes^*