Cis-acting region associated with lung cell-specific expression of the secretory leukoprotease inhibitor gene

Cis-acting Region Associated with Lung Cell-specific Expression of the Secretory Leukoprotease Inhibitor Gene

Toshiaki Kikuchi, Tatsuya Abe, Ken Satoh, Koh Narumi, Toshihiko Sakai, Shigefusa Abe, Satoshi Shindoh, Keiko Matsushima, and Toshihiro Nukiwa

Department of Respiratory Oncology and Molecular Medicine, Division of Cancer Control, Institute of Development, Aging and Cancer, Tohoku University, Sendai, Japan

Abstract

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Secretory leukoprotease inhibitor (SLPI) is a serine protease inhibitor, produced locally in respiratory and genital glands,but not in the liver. In the present study the promoter regionof this gene was analyzed to better understand the molecular mechanismsinvolved in transcriptional regulation. DNase-I hypersensitivesites were detected within 1 kbp upstream of exon I in chromatinstructures of type II pneumocyte cell line A549 and utero-cervicalcell line HeLa, both of which express SLPI mRNA transcripts. Thefunction of the SLPI promoter encompassing these DNase-I hypersensitivesites has been studied by deletion analysis with the luciferasegene as a transient expression vector. In this analysis, we foundthree transcription control regions that function in A549 cellsbut not in nonlung cell lines, such as HeLa and hepatoma Hep G2.Among three cis-regulatory regions, a proximal 41-bp region ( $-$ 132to $-$ 92 bp relative to the transcription start site) is responsiblefor the most striking magnitude of transcriptional activity. Thisregion corresponds to the transcriptional activating sequencedetected in another lung cell line, HS-24, indicating that this41-bp sequence is required for lung cell-specific expression.An electrophoretic mobility shift assay demonstrated that this41-bp promoter region contains an 11-bp recognition sequence fortwo nuclear binding proteins, one of which is abundant in lungcell lines, and the other in nonlung cell lines. These resultssuggest that the ratio of these two nuclear binding proteins confersthe cell type specificity on the expression pattern of the SLPIgene.

	Introduction

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Secretory leukoprotease inhibitor (SLPI) is a nonglycosylated serine protease inhibitor consisting of 107 amino acids (M_r11,726). Its major physiologic function is considered to be antineutrophilelastase protection at inflammatory sites (1). This serineprotease inhibitor has been demonstrated in several normal tissues,and produced and released into mucus by secretory cells in respiratory,genital, and lacrimal glands, but not in the liver, endocrineglands, or hematologic system (2). In the respiratory tract,SLPI was observed in alveolar type II epithelial cells, serouscells of submucosal glands, and nonciliated epithelial cells (2).

It was reported that SLPI gene expression in several lung epithelial cell lines is upregulated by phorbol ester (3), neutrophilelastase (4), corticosteroids (5), interleukin (IL)-1 $beta$ ,and tumor necrosis factor- $alpha$ (TNF- $alpha$ ) (6). The stimulatory effectof phorbol ester is mediated by changes in gene transcriptionand mRNA stability (3). Moreover, it was found that up to 1.3kilobase pair (kbp) of the 5' flanking sequence was transcriptionallyactive in human lung carcinoma cell lines, supporting the conceptthat this promoter region contains cis-active elements necessaryfor SLPI gene expression (7). However, little is known aboutthe tissue-specific transcriptional regulation of the SLPI gene,nor has the interaction between cis-acting sequences and nuclearfactors required for the regulatory pathway been demonstrated.

In the present study, using the transiently expressed reporter gene assay as well as DNase-I hypersensitive mapping, we definethe cis-acting region that activates SLPI gene transcription onlyin human lung epithelial cell lines. Within this lung cell-specificregulatory region, we further reveal an 11-bp recognition sequence, $-$ 102 to $-$ 92 bp upstream of the transcription start site, for twonuclear proteins. Because one of the binding proteins is abundantin lung cell lines and another in nonlung cell lines, the ratioof these two nuclear factors is likely to be critical for celltype-specific transcription of the SLPI gene.

	Materials and Methods

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Cell Culture

Human lung adenocarcinoma A549 cells, human utero-cervical carcinoma HeLa cells, and human hepatocellular carcinoma Hep G2cells were distributed by the Cancer Cell Repository (Tohoku University,Sendai, Japan). Human lung squamous cell carcinoma HS-24 cellswere provided by Dr. W. Ebert (Thoraxklinik der LVA Baden, Heidelberg-Rohrbach,Germany). Cells were cultured as a monolayer in Dulbecco's modifiedEagle's medium (DMEM; GIBCO-BRL, Gaithersburg, MD) supplementedwith 10% fetal calf serum (FCS) at 37°C in a humidified 5% CO₂atmosphere.

RNA Isolation and Northern Blot Hybridization

Total cellular RNA was isolated from cultured cells by acid guanidinium thiocyanate-phenol chloroform extraction (8), andpoly(A)⁺ RNA was prepared from total cellular RNA by oligo(dT)-cellulosecolumn chromatography. Two micrograms of poly(A)⁺ RNA were electrophoresed on a 1% agarose gel containing 2.2 Mformaldehyde, and transferred to a nitrocellulose membrane. AcDNA probe was radiolabeled with [ $alpha$ -³²P]dCTP (~ 111 TBq/mmol) (Du Pont, Wilmington, DE) using the randomprimers DNA labeling system (GIBCO-BRL). Filter hybridizationwith the probe proceeded for 16 h at 68°C in hybridization buffercontaining 6× SSC, 5× Denhardt's solution, 0.5% sodium dodecylsulfate (SDS), and 100 µg/ml denatured fragmented salmon spermDNA. After hybridization, the membrane was washed successivelywith 2× SSC, 0.5% SDS at room temperature for 5 min with 2× SSC,0.1% SDS at room temperature for 15 min with 0.1× SSC, 0.5% SDSat 37°C for 1 h, and with 0.1× SSC, 0.5% SDS at 68°C for 1 h.The membrane was dried and exposed to a Fuji imaging plate (FujiPhoto Film Co., Minamiashigara, Japan). Scanning of the signalswas performed using a bio-imaging analyzer system (Fuji PhotoFilm Co.).

DNase-I Hypersensitive Site Mapping

Nuclei were prepared by homogenizing 108 cells in a glass Dounce homogenizer (Wheaton, Millville, NJ) with 15 strokes of aB pestle. The nuclei were resuspended in 1 ml of buffer A (10mM Tris-HCl [pH 7.4], 10 mM KCl, 3 mM MgCl₂), and 118 µl of thesuspension was treated with DNase I for each digestion time asfollows. Briefly, after adjusting the volume of the nuclear suspensionto 1 ml with buffer A, DNase I (Boehringer Mannheim Biochemicals,Indianapolis, IN) was added to a final concentration of 7.8 µg/ml.After incubation for 0 to 4 min at 30°C, digestion was stoppedby the addition of 100 µl of 5% SDS, and 125 mM EDTA, and 25 µlof proteinase K (10 mg/ml). Following overnight incubation at37°C, the DNA was purified by phenol-chloroform extraction andethanol precipitation. DNA (48 µg) from each sample was completelyrestricted with BamH I, electrophoresed on 1.2% agarose, and subjectedto Southern hybridization analysis using a ³²P-labeled DNA probe (pAK3) encompassing almost all of the intronI and exon II ([Pst I]-[BamH I] fragment; Figure 2a). The membranewas dried and analyzed by the bio-imaging analyzer system as usedfor Northern analysis.

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Figure 2. DNase-I hypersensitive site mapping in the SLPI gene. (a) Partial map of the SLPI gene and 5' flanking region with the sitesfor relevant restriction enzymes. Two BamH I sites are locatedin this area, one in exon II and the other 6 kbp upstream of exonII. DNase-I hypersensitive sites are evaluated within this 6-kbpBamH I genomic DNA fragment, using a 0.8-kbp (Pst I) (BamH I)probe (thick black line) corresponding to +140 ~ +961 bp downstreamof the transcription start site. Four DNase-I hypersensitive sites(DH1, DH2, DH3, and DH4) detected in both A549 and HeLa cellsare indicated with arrows. (b) Southern analysis demonstratingDNase-I hypersensitive sites in the chromatin of HeLa cells. Nucleiisolated from HeLa cells were treated with DNase I for the timeperiods indicated (top). The DNA was extracted, digested withBamH I, and analyzed by Southern blot hybridization with a 0.8-kbp(Pst I) (BamH I) probe (a). The parental fragment and four distinctfragments liberated by DNase-I digestion (DH1, DH2, DH3, and DH4)are indicated by arrows, with the sizes in kilobase pairs withinparentheses.

Construction of Luciferase Expression Vector

The serially deleted fragments of the SLPI promoter were synthesized by polymerase chain reaction (PCR) using AmpliTaq (Perkin-ElmerCetus, Norwalk, CT), with appropriate forward primers, a commonreverse primer, and plasmid pAK2 as template, pAK2 is a pGEM-4Z(Promega, Madison, WI) with an inserted 1.2 kbp of the 5' flankingregion of the SLPI gene ( $-$ 1,228 to +145 bp relative to the transcriptionstart site) (9). A Kpn-I site was created near the 5' end ofeach forward primer, and an Xho-I site was created near that ofthe reverse primer (10). The PCR product was digested with bothKpn I and Xho I and inserted into the polylinker region of thepGL2-Basic (Promega), keeping the direction of the promoter upstreamof the firefly luciferase gene. The sequence of each constructwas confirmed by the dideoxy chain-termination method (11) withSequenase version 2.0 (United States Biochemical Corp., Cleveland,OH).

Transfection, Luciferase Assay, and Chloramphenicol Acetyltransferase Assay

Cells were transfected by the calcium phosphate technique (12) as follows. Twenty-four hours prior to transfection, A549and HeLa cells were seeded onto plastic dishes (9 cm in diameter)at a density of 1 × 10⁶/plate, and Hep G2 cells at a density of 4 × 10⁶/plate. Twenty micrograms of the luciferase construct and 5 µgof pRSVcat, in which the coding region of the chloramphenicolacetyltransferase (CAT) gene is ligated to the long terminal repeatof the Rous sarcoma virus (13), were coprecipitated and lefton the cells for 4 h. The cells were then exposed to 15% glycerolfor 30 s (HeLa cells) or 2 min (A549 and Hep G2 cells), and refedwith growth medium. Cells were harvested 48 h after transfection,and divided into equal aliquots for luciferase and CAT assays.For the luciferase assay (14), pelleted cells were lysed in250 µl of 25 mM Tris-phosphate (pH 7.8), 2 mM dithiothreitol (DTT),2 mM 1,2-diaminocyclohexane-N,N,N',N'-tetraacetic acid, 10% glycerol,and 1% Triton X-100, and incubated for 15 min at room temperature.The cell-free extract prepared by centrifugation was analyzedfor luciferase activity by a luminometer Lumat LB 9501 (Berthold,Berlin, Germany). The reaction was started by mixing 20 µl ofthe cell extract with 100 µl of assay buffer (Toyo Ink Mfg. Co.,Tokyo, Japan), which was composed of 20 mM Tricine, 1.07 mM (MgCO₃)₄Mg(OH)₂·5 H₂O, 2.67 mM MgSO₄, 0.1 mM EDTA, 33.3 mM DTT, 270 µM coenzymeA, 470 µM luciferin, and 530 µM ATP. Light emission was measuredfor 10 s after starting the reaction, and integrated over timeby the luminometer. The value was corrected after protein quantificationof the extract according to the method of Bradford (15). Luciferaseactivity was assayed within the linear range in terms of the reactiontime and the amount of the enzyme. To monitor the transfectionefficiency for each dish, the CAT activity was assayed as describedby Gorman and colleagues (16). Following standardization withthe acetylation ratio of [¹⁴C]chloramphenicol, the level of luciferase activity in each samplewas normalized relative to the activity of p-1228LUC plasmid inA549 cells. The result was expressed as the mean ± SEM of threeindependent transfections for each construct. Statistical comparisonbetween a construct and the subsequently truncated construct wasmade by a two-tailed Student's t test, and a value of P < 0.01was accepted as indicating statistical significance.

Preparation of Nuclear Extracts

Nuclear extract was prepared as described by Schreiber and colleagues (17). Cells (3.5 to 4.5 × 10⁶) were washed with phosphate-buffered saline (PBS), and resuspendedin 400 µl of buffer A (10 mM Hepes [pH 7.8], 10 mM KCl, 0.1 mMEDTA, 2 mM DTT, 1 mM phenylmethylsulfonyl fluoride [PMSF]). Thecells were incubated on ice for 15 min, then 25 µl of 10% NonidetP-40 (NP-40) was added, and the tube was vigorously vortexed for10 s. The homogenate was centrifuged for 30 s in a microcentrifuge,and the nuclear pellet was resuspended in 50 µl of buffer C (20mM Hepes [pH 7.8], 420 mM NaCl, 5 mM EDTA, 5 mM DTT, 1 mM PMSF,10% glycerol). The tube was vigorously rocked at 4°C for 30 minon a shaking platform, and centrifuged in a microfuge for 10 min.The supernatant was frozen in aliquots at $-$ 70°C. Protein concentrationwas determined by the method of Bradford (15), using the proteinassay dye reagent provided by Bio-Rad Laboratories (Richmond,VA) with bovine serum albumin as a standard.

Electrophoretic Mobility Shift Assay

A duplex oligonucleotide probe was labeled with [ $alpha$ -³²P] dATP (~ 222 TBq/mmol)(Du Pont) by filling in a 5' overhanging end withKlenow DNA polymerase. The end-labeled probe (~ 0.5 ng of DNA)was incubated in the binding reaction buffer (10% glycerol, 5mM Tris-HCl [pH 7.5], 25 mM NaCl, 0.25 mM DTT, 0.05% NP-40) with0.3 µg of poly(dI-dC) · poly(dI-dC) and 3 µg of a crude nuclearextract for 20 min at room temperature. Following the bindingreaction, the mixture was electrophoresed through a low ionicstrength gel (5% polyacrylamide, 7 mM Tris-HCl [pH 7.5], 3 mMsodium acetate, 1 mM EDTA). Electrophoresis was carried out at10 V/cm for 2.5 h. The gel was dried and analyzed by the bio-imaginganalyzer system as used for Northern analysis. For a competitionexperiment, 20 ng of specific or nonspecific competitor DNA wasincubated in the mixture prior to addition of the labeled probe.

	Results

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Expression of the SLPI Gene in A549 and HeLa Cells

Northern analysis revealed that the poly(A)⁺ RNA prepared from A549 and HeLa cells contained 0.7-kb RNA transcripts that hybridizedwith the SLPI cDNA, but no band was detected when Hep G2 cellswere used (Figure 1). The amount of SLPI mRNA transcripts is lessabundant in type II pneumocyte cell line A549 as compared withthe utero-cervical cell line HeLa. The entirety of the mRNA wasconfirmed using a glyceraldehyde-3-phosphate dehydrogenase (GAPDH)cDNA probe, even with hepatocyte cell line Hep G2, which showedundetectable SLPI mRNA transcripts.

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Figure 1. Expression of the secretory leukoprotease inhibitor (SLPI) gene in human epithelial cell lines. Shown is the result of Northernanalysis of the poly(A)⁺ RNA isolated from Hep G2 cells, A549 cells, and HeLa cells. Twomicrograms of poly(A)⁺ RNA was loaded on each lane, electrophoresed on a 1.0% agarosegel containing 2.2 M formaldehyde, and blotted onto nitrocellulosemembrane. The membrane was hybridized with a labeled probe ofSLPI cDNA or GAPDH cDNA followed by autoradiography. Althoughpoly(A)⁺ RNA from each cell line contains a similar amount of GAPDH transcriptswith a size of 1.4 kb, SLPI transcripts with a size of 0.7 kbwere detected in poly(A)⁺ RNA from A549 cells and HeLa cells but not in that from Hep G2cells.

Mapping of DNase-I Hypersensitive Sites

In chromatin analysis, four DNase-I hypersensitive sites were identified in a 6-kbp BamH I restriction endonuclease area containingthe first exon of the SLPI gene (Figure 2a). Using a 0.8-kbp (PstI)-(BamH I) probe (+140 to +961 bp downstream of the transcriptionstart site), four DNA fragments (1.5, 1.2, 1.0, and 0.7 kbp),were detected in Southern analysis of DNase-I digested HeLa nuclei(Figure 2b). In the context of the SLPI gene structure, correspondingDNase-I hypersensitive sites, designated DH1 to DH4, were located0.6, 0.3, and 0.1 kbp upstream from the beginning of exon I, andwithin the first intron. These four DNase-I hypersensitive siteswere also observed with nuclei prepared from A549 cells (datanot shown). This result suggests that candidates as cis-regulatoryelements are likely to lie within 1 kbp upstream of the SLPI gene.

Functional Analysis of the SLPI Promoter

Evaluation of the SLPI promoter by reporter gene assay encompassing DNase-I hypersensitive sites. When the luciferase reportergenes with various lengths of the SLPI promoter region were constructedand evaluated, the 5' flanking region of the SLPI gene from $-$ 1,228to +22 bp is sufficient to direct transcription in a cell type-specificmanner. The longest SLPI promoter region from $-$ 1,228 to +22 bp(p-1228LUC) yielded 125-fold and 185-fold greater luciferase activitiesthan pGL2-Basic in SLPI-expressing cell lines, A549 and HeLa cells,respectively (Figure 3). In contrast, transfection of this construct(p-1228LUC) into Hep G2 cells supported only slight luciferaseactivity above that of the promoterless vector (pGL2-Basic). Theseresults are consistent with the transcriptional activity or inactivityof the SLPI gene assessed by Northern blot analysis.

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Figure 3. Transient transfection analysis of the SLPI promoter in A549, HeLa, and Hep G2 cells. On the left is shown a 5' deletion series.Various lengths (up to $-$ 1,228 bp relative to the transcriptionstart site) of the SLPI promoter and the first exon comprising22 bp of the 5' untranslated region were linked upstream of theluciferase gene (LUC). The numbers to the left of each constructindicate the 5' end point. These constructs and a plasmid lackinga promoter (pGL2-Basic) were transiently transfected into A549,HeLa, and Hep G2 cells, and the luciferase activities were assayed.On the right is listed the relative luciferase activity of eachconstruct expressed as a percentage of the activity of p-1228LUCin A549 cells (see MATERIALS AND METHODS for details). The valuesrepresent the mean ± SEM of three independent transfections. Asterisksdenote significant differences (P < 0.01) compared with the subsequentlytruncated construct.

Deletion analysis of the sequence flanking the SLPI promoter. Transfection of fusion genes composed of sequentially deletedSLPI promoter and a luciferase reporter gene into A549 cells provedthat three distinct regions are concerned in the promoter function(Figure 3). Luciferase activity varied significantly in A549 cellswith truncations from p-1059LUC (2-fold activation), p-849LUC(3-fold reduction), and p-132LUC (12-fold reduction), while activityremained constant in both HeLa and Hep G2 cells. These data indicatethat three distinct cis-acting elements that function only inA549 cells lie in the 5' flanking region of the SLPI gene, andthat no specific segment from $-$ 1228 to $-$ 92 bp affects SLPI transcriptionin either HeLa or Hep G2 cells.

Similar deletion analysis previously demonstrated that the SLPI promoter spanning $-$ 115 to $-$ 97 bp is essential for constitutiveand phorbul myristate acetate (PMA)- induced SLPI expression inhuman squamous lung carcinoma HS-24 cells (3). Among threeA549-restricted regulatory regions revealed in our deletion study,the most proximal region from $-$ 132 to $-$ 92 bp not only correspondsto the cis-acting region detected in HS-24 cells, but also isresponsible for the striking magnitude (12-fold) of transcriptionalactivation in A549 cells. These observations suggest that this41-bp promoter sequence ( $-$ 132 to $-$ 92 bp) shares cis-acting elementsassociated with lung cell-specific expression of the SLPI gene.

Binding of Nuclear Proteins to the SLPI Promoter

A DNA-protein interaction assay using A549 nuclear extracts revealed that two nuclear proteins interact with the lung cell-specificpromoter ( $-$ 132 to $-$ 92 bp) in a sequence-specific manner (Figures4 and 5). In the analysis, two DNA-protein complexes, termed SLPI-B1and SLPI- B2, were detected (Figure 5, lane 2). The formationof SLPI-B1 and SLPI-B2 complexes was diminished by competitionwith excess unlabeled specific competitor S (Figure 4, lane 3),but was not diminished by competition with excess unlabeled nonspecificcompetitor (Figure 4, lane 4), demonstrating the sequence specificityof these two DNA- protein interactions.

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Figure 4. The nucleotide sequence of the 5' flanking region and first exon of the SLPI gene. The numbering indicates the nucleotideposition relative to the transcription start site, which is designatedas +1. Coding sequence for amino acids (boldface) begins +23 bpdownstream. The CAAT ( $-$ 88 to $-$ 84 bp) and TATA ( $-$ 27 to $-$ 22 bp)boxes are also indicated. Schematic representation of the duplexoligonucleotides used in the electrophoretic mobility shift assay(EMSA) is inserted. The positions of the 41-bp specific competitor(S) and three short duplex oligonucleotides (DO1, DO2, and DO3)are indicated.

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Figure 5. EMSA analysis of the 41-bp lung cell-specific SLPI promoter sequence corresponding to competitor S. Nuclear extract from A549cells (A549 NE) was prepared as described in MATERIALS AND METHODS.Three micrograms of nuclear protein was incubated with the ³²P-labeled 41-bp DNA probe ( $-$ 132 to $-$ 92 bp). Protein-DNA complexeswere resolved by electrophoresis on a 5% polyacrylamide gel. Twospecific DNA-protein complexes, SLPI-B1 and SLPI-B2, are indicatedby arrows on the right. Lane 1, without nuclear extract; lane2, with nuclear extract in the absence ( $-$ ) of competitor (Comp.);lane 3, with nuclear extract in the presence of the 41 bp-specificcompetitor S ( $-$ 132 to $-$ 92 bp); lane 4, with nuclear extract inthe presence of nonspecific competitor NS. As a nonspecific competitor,the 41-bp duplex oligonucleotide without homology to the specificcompetitor S was used.

SLPI-B1 and SLPI-B2 Complexes among Epithelial Cell Lines

Although SLPI-B1 and SLPI-B2 complexes were seen in the cell lines used, the signal intensity varied according to the SLPIpromoter function of the cell type (Figure 6). In this context,when using nuclear extracts from lung cell lines (HS-24 or A549cells) in which the 41-bp SLPI promoter region ( $-$ 132 to $-$ 92 bp)is transcriptionally active, the SLPI-B1 complex is much moreabundant than the SLPI-B2 complex (Figure 6, lanes 3 or 4). Incontrast, when using nuclear extract from nonlung cell lines (HepG2 or HeLa cells) in which the 41-bp promoter region is transcriptionallyinactive, the SLPI-B2 complex is dominant over the SLPI-B1 complex(Hep G2 cells; Figure 6, lane 1) or as abundant as the SLPI-B1complex (HeLa cells, Figure 6, lane 2). This experimental evidencesuggests that the ratio of SLPI-B1 and SLPI-B2 binding proteinshas important implications for cell type-specific function ofthis 41-bp SLPI promoter sequence.

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Figure 6. Analysis of nuclear protein-DNA complexes of SLPI- B1 and SLPI-B2 in several epithelial cell lines. The ³²P-labeled 41-bp DNA probe ( $-$ 132 to $-$ 92 bp) was incubated with3 µg of nuclear extracts (NE) from Hep G2 (lane 1), HeLa (lane2), HS-24 (lane 3), and A549 cells (lane 4). The reaction mixturewas resolved on a 5% polyacrylamide gel. Relative binding of SLPI-B1and SLPI-B2 are indicated at the bottom. ++, Strong; +, weak.

Sequence Requirements of SLPI-B1 and SLPI-B2 Complexes

Another DNA competition assay revealed that the 11-bp sequence within the 41-bp lung cell-specific promoter region is indispensablefor the formation of SLPI-B1 and SLPI-B2 complexes (Figure 7).To evaluate the sequence requirements of SLPI-B1 and SLPI-B2,HeLa cells expressing abundant SLPI-B1 and SLPI-B2 binding proteins(Figure 6, lane 2) were used in this competition assay. Nuclearextract was preincubated with an excess amount of a cold shortcompetitor (DO1, DO2, and DO3; Figure 4), and an electrophoreticmobility shift assay (EMSA) was performed with the ³²P-labeled 41-bp probe ( $-$ 132 to $-$ 92 bp). As a result, using oligonucleotideDO1 ( $-$ 132 to $-$ 113 bp) and DO2 ( $-$ 122 to $-$ 103 bp) as the cold competitor(Figure 7, lanes 4 and 5), a pattern similar to that of the nonspecificcompetitor NS (Figure 7, lane 3) in the formation of SLPI-B1 andSLPI-B2 complexes was observed, indicating that the DNA sequencebetween $-$ 132 and $-$ 103 bp is not responsible for the DNA-proteinbinding. However, when oligonucleotide DO3 ( $-$ 112 to $-$ 92 bp) wasused as the competitor, the formation of both SLPI-B1 and SLPI-B2complexes was strongly suppressed (Figure 7, lane 6). These datademonstrate that both SLPI- B1 and SLPI-B2 binding proteins interactwith the identical sequence in DO3 but not in DO1 and DO2. A short11-bp promoter sequence, from $-$ 102 to $-$ 92 bp, is likely to bea target sequence for these nuclear proteins in a mutual interactivemanner.

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Figure 7. Comparison of complex formation with partial specific competitors. EMSA competition experiment was performed as describedin MATERIALS AND METHODS. The ³²P-labeled 41-bp DNA probe ( $-$ 132 to $-$ 92 bp) and HeLa cell nuclearextract were incubated with or without competitor (Comp.). Lane1, in the absence of competitor; lane 2, in the presence of the41 bp-specific competitor S ( $-$ 132 to $-$ 92 bp); lane 3, in the presenceof nonspecific competitor NS; lanes 4-6, in the presence of shortspecific competitors DO1, DO2, and DO3. Relative binding of SLPI-B1and SLPI-B2 are indicated at the bottom. ++, Strong; ±, barelydetectable; $-$ , undetectable.

	Discussion

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To provide a basic framework for understanding the shared mechanisms of gene regulation in respiratory epithelial cells, transcriptionalelements in the surfactant protein (SP) (A, B, and C) and Claracell secretory protein (CCSP) have been analyzed. Concerning theSP-B gene, $-$ 218 bp from the transcription start site is sufficientto confer lung epithelial cell gene expression in vitro, and thyroidtranscription factor 1 (TTF-1) and hepatocyte nuclear factor 3/forkhead(HNF-3/fkh) family members bind to and activate the SPB-f1 site( $-$ 113 to $-$ 90 bp) and SP-B-f2 site ( $-$ 91 to $-$ 70 bp), respectively(18, 19).

The essential process that regulates the lung cell-specific expression of the SLPI gene was shown, using cultured cell lines(9), to occur during transcription in vitro. Moreover, Maruyamaand colleagues have demonstrated, using transient transfectionof lung cancer-derived HS-24 cells, that a positive cis-activeelement is located between $-$ 115 and $-$ 97 bp relative to the transcriptionstart site (3). However, little information is available foridentification of transcriptional motifs controlling the SLPIgene expression, and nuclear proteins from lung cells have notbeen shown to bind the regulatory cis elements.

In this study, we have examined the mechanisms for the lung epithelium-specific transcription of the SLPI gene, focusing oncis-acting regions in the promoter and nuclear proteins interactingwith the sequences. By transient luciferase expression assay,we identified three cis-acting regulatory regions functioningspecifically in lung cell line A549. Among these three regions,the most proximal sequence (from $-$ 132 to $-$ 92 bp) is responsiblefor the most striking magnitude of transcriptional activationin A549 cells. This region contains the promoter sequence from $-$ 115 to $-$ 97 bp, which was reported to share the transcriptionalregulatory elements in HS-24 cells (3). Thus, we consider the41-bp promoter region from $-$ 132 to $-$ 92 bp to be associated withlung cell-specific transcription of the SLPI gene. Analysis byEMSA of this 41-bp promoter sequence indicates that two nuclearfactors, SLPI-B1 and SLPI-B2 binding proteins, interact with theshort sequence from $-$ 102 to $-$ 92 bp in a sequence-specific manner.Furthermore, when using nuclear extract of A549 or HS-24 cells,in which the 41-bp promoter sequence is shown to be requisitefor the transcriptional activation by the transient transfectionassay, the nuclear protein-DNA complex of SLPI-B1 is much moreabundant than that of SLPI-B2 (Figure 6, lanes 3 and 4). Conversely,when using nuclear extract of Hep G2 or HeLa cells, in which deletionof the 41-bp promoter sequence made no change in terms of transcriptionalactivity, the nuclear protein-DNA complex of SLPI-B2 is much moreabundant than that of SLPI-B1 (Hep G2 cells) or is as abundantas that of SLPI-B1 (HeLa cells) (Figure 6, lanes 1 and 2). A hypotheticalinterpretation of these results is as follows: in pulmonary epithelialcells such as A549 and HS-24 cells, abundant SLPI-B1 binding proteininteracts with the 11-bp promoter sequence, and this binding providescrucial signals required for the activation of the transcriptionalunit of the SLPI gene. In contrast, in nonlung cell lines suchas Hep G2 and HeLa cells abundant SLPI-B2 binding protein dominatesthe 11-bp promoter sequence, and inactivates the cis-acting sequenceby interacting with the binding of the positively acting SLPI-B1nuclear protein.

It is interesting to note that this 11-bp promoter sequence contains the sequence 5' CGTTTCC 3' ( $-$ 102 to $-$ 96 bp; Figure 4),which shows homology (five of seven nucleotides match) to thecore sequence T(G/A)TTTA(C/ T) found in the binding site for anumber of HNF-3/fkh families (20). The consensus HNF-3 bindingsite (22), centered around the HNF-3/fkh core sequence, hasbeen identified in the SP-A (23), SP-B (24), and CCSP (25,26) promoters, and it has been suggested that HNF-3 proteinsare likely to play a critical role in regulating the expressionof these genes in the lung. Despite an agreement of the SLPI promotersequence ( $-$ 105 to $-$ 94 bp) with the consensus HNF-3 binding sitesequence (8 of 12 nucleotides match), the binding motif of anyknown HNF-3/fkh family members so far does not completely correspondto this SLPI promoter sequence. Sequence variations in the coreand flanking sequence suggest that as yet unidentified HNF-3/fkhfamily members may also be implicated in SLPI promoter function.Future experiments will be required to identify these nuclearfactors.

In summary, we have identified the lung cell-specific regulatory region in the SLPI promoter, and have shown that the amountof two nuclear proteins interacting with this regulatory sequenceis different between lung and nonlung cell lines. The identificationand characterization of these proteins should further our understandingof the molecular mechanisms of SLPI gene regulation.

	Footnotes

Address correspondence to: Toshiaki Kikuchi, Department of Respiratory Oncology and Molecular Medicine, Division of Cancer Control, Institute of Development, Aging and Cancer, Tohoku University, 4-1 Seiryo- machi, Aoba-ku, Sendai 980, Japan. E-mail: kikuchi{at}idac.tohoku.ac.jp

(Received in original form April 16, 1995 and in revised form January 13, 1997).

Acknowledgments: The authors thank Dr. Masakichi Motomiya for his helpful advice, which prompted the start of the present study; and also Drs.Masanori Terajima and Ikuko Sagami, for their invaluable commentsin designing the experimental protocols.

This work was supported in part by a grant from the Ministry of Education, Science, and Culture of Japan (No. 08670646).

Abbreviations CAT, chloramphenicol acetyl transferase; DTT, dithiothreitol; EMSA, electrophoretic mobility shift assay; GAPDH, glyceraldehyde-3-phosphate dehydrogenase; SLPI, secretory leukoprotease inhibitor; SDS, sodium dodecyl sulfate.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

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2. Franken, C., C. J. Meijer, and J.H. Dijkman. 1989. Tissue distributionof antileukoprotease and lysozyme in humans. J.Histochem. Cytochem. 37: 493-498 [Abstract].

3. Maruyama, M., J. G. Hay, K. Yoshimura, C.S. Chu, and R. G. Crystal. 1994. Modulationof secretory leukoprotease inhibitor gene expression in humanbronchial epithelial cells by phorbol ester. J.Clin. Invest. 94: 368-375 .

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