1Interdepartmental Nutrition Program, Purdue University, West Lafayette, Indiana 47907; 2Institute National de la Sante et de la Recherche Medicale, Unite 381, 67200 Strasbourg, France; 3Division of Gastroenterology and Nutrition, Department of Medicine, Children's Hospital, and Department of Pediatrics, Harvard Medical School, Boston, Massachusetts 02115; and 4Dorothy R. Friedman School of Nutrition Science and Policy, Tufts University, Boston, Massachusetts 02111
Submitted 19 March 2004 ; accepted in final form 21 June 2004
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ABSTRACT |
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intestine; enterocyte; 1,25 dihydroxyvitamin D
One such gene encodes calbindin D9k, an EF hand calcium-binding protein critical for calcium absorption that is expressed in the duodenum and cecum of rodents (5, 7). The expression of calbindin D9k is regulated by the hormonally active form of vitamin D, 1,25 dihydroxyvitamin D [1,25(OH)2 D] (7, 22, 47). Whereas previous reports have identified putative vitamin D response elements in the calbindin D9k promoter from various species (12, 28, 45), other data suggest that posttranscriptional regulation may be a more important mode of calbindin D9k regulation by 1,25(OH)2 D (14, 15, 23, 46). In addition to vitamin D regulation, calbindin D9k expression is restricted to the differentiated villus compartment (24, 38, 49, 53), indicating that it is under the control of factors programming intestinal cell differentiation; mutation of a cdx-2 response element at 3.5 kb decreased the intestinal expression of a calbindin D9k reporter gene construct by 99% in transgenic mice (9). Several other potential regulatory sites in the proximal rat calbindin D9k promoter have been reported on the basis of footprinting and gel-shift assays (1, 34), i.e., a proximal cdx-2 element and sites for HNF-1, HNF-4, and CCAAT enhancer binding protein (C/EBP). None of those sites has been assigned a functional role in the regulation of calbindin D9k promoter activity.
Here we characterized 1,25(OH)2 D- and differentiation-mediated regulation of the human calbindin D9k gene promoter in Caco-2 cells, an in vitro model for small intestinal differentiation (2, 13, 18, 51). Our findings demonstrate that the calbindin D9k gene is poorly regulated at the transcriptional level by 1,25(OH)2 D but strongly upregulated during spontaneous differentiation to an enterocyte-like phenotype. Two HNF-1 binding sites, one at 98 and a novel, distal HNF-1 binding site at 3131 are essential for the differentiation-dependent expression of calbindin D9k. In addition, our findings suggest that cdx-2 is a permissive factor that influences the basal expression level and that HNF-1-mediated transcriptional regulation of the calbindin D9k promoter requires a complex interaction between the proximal and the distal HNF-1 response element.
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MATERIALS AND METHODS |
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Unless otherwise noted, all chemicals were obtained from Fisher Scientific (Fair Lawn, NJ), the media and supplements were purchased from Sigma (St. Louis, MO), and tissue culture plates were purchased from Corning Costar (Cambridge, MA).
The parental strain of Caco-2 cell (HTB-37) and the BBe clone (CRL-2102) were obtained from American Type Culture Collection (Rockville, MD). TC7 cells were first described by Chantret et al. (6). These were provided to us at passage 69 by Dr. Mark Failla (Ohio State University). Cells were cultured as previously described (20). The BBe and TC7 clones were used because they have previously been demonstrated to develop a more differentiated phenotype (e.g., higher sucrase activity) compared with the parental line (6, 42). To ensure that the cell lines would reach confluence concurrently (4 days in culture), different seeding densities were used for each cell line, i.e., parental Caco-2, BBe, and TC7 cells were seeded onto six-well dishes at a density of 128,000, 256,000, and 64,000 cells/well, respectively. For transfection experiments, TC7 cells were seeded onto 24-well dishes at a density of 15,000 cells/well.
Regulation of Calbindin D9k Expression by 1,25(OH)2 D and Spontaneous Differentiation
Spontaneous differentiation. Parental Caco-2, BBe, and TC7 cells were grown in culture until 50% confluent (2 days in culture), confluent (4 days in culture), 4 days postconfluent (8 days in culture), and 11 days postconfluent (15 days in culture). At each time point, cells (n = 3 wells per cell line) were harvested into 1 ml TriReagent (Molecular Research Center, Cincinnati, Ohio), total RNA was isolated following the manufacturer's directions, and specific messages were assessed by RT-PCR. The experiment was repeated twice (n = 6 per time point per cell line).
To evaluate whether the expression of calbindin D9k mRNA was transcriptionally activated during spontaneous differentiation, expression of a full-length calbindin D9k promoter reporter gene construct (CaBP4600) was examined under two protocols. In one study, proliferating cultures of TC7 cells were transfected and then harvested at 50% confluent, 5 days in culture (1 days postconfluent), 9 days in culture (5 days postconfluent), and 13 days in culture (9 days postconfluent). In the second study, 2- or 9-day cultures of BBe and TC7 cells were transiently transfected and studied 24 h later. This second protocol was utilized for all subsequent experiments. Cells were either seeded onto six-well dishes (for the study of proliferating cells) or 24-well dishes (for the study of postproliferative cultures) and transfected with the Lipofectamine Plus reagent (Invitrogen, Carlsbad, CA). Briefly, 2 µg of the specific experimental vector was cotransfected along with a Renilla-expressing control vector, pRL-CMV (Promega, Madison, WI; molar ratio between the experimental and control vector = 250:1). In proliferating cells, transfection medium was replaced with 10% FBS DMEM 2 h after transfection. For differentiated cells, an equal volume of 20% FBS DMEM was added to each well 8 h after transfection, and new medium was added at 24 h. The prolonged exposure of differentiated cells to plasmid was necessary to overcome the low transfection efficiency we observed in these tight monolayers of nonproliferating cells. Cells were harvested, and luciferase activity was measured with the Dual-Luciferase Reporter Assay System (Promega, Madison, WI) in a luminometer (model TD-20/20; Twin Designs, Sunnyvale, CA). The firefly luciferase activity (experimental plasmid) was normalized to Renilla luciferase activity (control plasmid) to control for variability in transfection efficiency. All treatments were examined in triplicate, and each experiment was conducted at least twice.
1,25(OH)2 D treatment. TC7 cells were seeded into six-well dishes and cultured for 2, 8, or 15 days. Cells were treated with either 100 nM 1,25(OH)2 D or ethanol vehicle (0.1% final concentration) for 48 h and then harvested for the examination of gene expression by RT-PCR.
Transcriptional regulation of the CaBP4600 construct was examined in 13-day cultures of TC7 cells. Cells were transiently transfected with either the CaBP4600 construct or a rat 24-hydroxylase promoter reporter construct provided to us by Dr. John Omdahl (30). Twenty-four hours after the transfection, cells were treated with 100 nM 1,25(OH)2 D for 24 h, and promoter activity was assessed after an additional 24 h as described above. For both natural and reporter-gene studies, the treatments were examined in triplicate and each experiment was conducted twice.
RT-PCR analysis.
Levels of specific messages were assessed by RT-PCR as described previously (21, 22). PCR primers used were sucrase (GenBank accession no. X63597): forward, 5'-GGTGGTCACATCCTACCATGTCAAG-3', reverse, 5'-CTGGGATATCTTTTTACTAA-3' (annealing temperature = 55°C); calbindin D9k (GenBank accession no. X65869): forward, 5'-ATGAGTACTAAAAAG-TCTCCT-3', reverse, 5'-CTGGGATATCTTTTTTACTAA-3' (annealing temperature = 55°C); cdx-2 (GenBank accession no. U51096): forward, 5'-AGCCAAGTGAAAACCAGGAC-3', reverse, 5'-CAGGGACAGAGCCAGACAC-3' (annealing temperature = 55°C); GAPDH (GenBank accession no. X02231): forward, 5'-CCATACAGGCAGCTTCGG-3', reverse, 5'-AGTCATCCACGAG-CGATTTG-3' (annealing temperature = 55°C); Pdx-1 (GenBank accession no. U35632): forward, 5'-GCCGCATGAAGTGGAAA-AAGG-3', reverse, 5'-TGTGGCGACGCGCTTAAGG-3' (annealing temperature = 55°C); HNF-1 (GenBank accession no. NM_000545): forward, 5'-TAGTGGAGGAGTGCAACAGGGC-3', reverse, 5'-TGGGAGAACTGGACGGGCTG-3', (annealing temperature = 60°C); HNF-1
(GenBank accession no. NM_000458): forward, 5'-GATGCCCACACACCACTTAC-3', reverse, 5'-TACGGCTTTCTTGCTTCCTC-3' (annealing temperature = 57°C); C/EBP
(GenBank accession no. XM009180): forward, 5'-CCCGAGTCACACCAGAAAG-3', reverse, 5'-CCGAGCAAAACCAAAACAA-3' (annealing temperature = 57°C). All PCR reactions used the cycling conditions of 94°C for 15 s and primer annealing temperature for 1 min 30 s, and 72°C for 45 s. PCR cycle numbers used were sucrase-isomaltase (27 cycles), cdx-2 (27 cycles), GAPDH (17 cycles), calbindin D9k (2 and 4 days = 35 cycles; 8 days = 27 cycles for BBe and P, 23 cycles for TC7, 15 days = 27 cycles for BBe and P; 21 cycles for TC7), HNF-1
(28 cycles), HNF-1
(24 cycles), C/EBP
(27 cycles), and Pdx-1 (35 cycles). These cycles were chosen so that the amplification was conducted in the linear range of amplification efficiency for each of the primer sets (data not shown). The resulting PCR products were subjected to electrophoresis on 2.5% agarose gels containing ethidium bromide, and bands were visualized under UV light. Gel data were recorded by using the Bio-Rad FluorS Imaging System, and relative densities of the bands were determined by using Quantity One software (Bio-Rad laboratories, Hercules, CA). Data were normalized for the expression of GAPDH within the sample. For calbindin D9k, we adjusted the data to account for differences in cycle numbers using the equation An = Ao(1 + R)n to determine a correction factor [where An = the amount of product produced at n cycles, Ao = the starting amount of cDNA, R = the amplification efficiency (assumed to be 0.8), and n = the cycle number]. Use of this correction factor permitted us to compare the transcript levels for calbindin D9k across time and between cell lines.
In Silico Analysis of the Calbindin D9k Gene Promoter
A computer-based comparison of the calbindin D9k gene promoter from mouse, rat, and human was conducted by using sequences available in GenBank (rat = GenBank accession no. X16635; mouse = GenBank accession no. AY034822 submitted from our laboratory; human = GenBank accession nos. X13042 and AL445467). The Compare (16 bp/21 bp window homology match) and DotPlot programs (GCG, Madison, WI) were used to identify promoter regions (clusters) with high cross-species sequence homology. These conserved clusters were examined for potential response elements using the computer program SIGSCAN (Advanced Bioscience Computer Center of The National Institutes of Health, http://bimas.dcrt.nih.gov/molbio/signal/) and the mammalian response element database TRANSFAC (54). When a putative response element was identified in the human calbindin D9k promoter, we examined the rat and mouse promoters to determine whether the element was conserved in these species.
Deletion-Mutation and Transcription Factor Activation Studies of the Human Calbindin D9k Gene Promoter
TC7 cells were either seeded onto six-well dishes (for the study of proliferating cells) or 24-well dishes (for the study of postproliferative cultures) and transfected with various constructs containing deletions of large promoter regions or mutations of specific response elements. Analysis of promoter activity was conducted as described earlier in Spontaneous differentiation. All treatments were examined in triplicate, and each experiment was conducted at least twice. In other experiments, proliferating cultures of TC7 or HeLa cells were transiently transfected with the CaBP4600 construct in the presence or absence of expression vectors for mouse cdx-2, HNF-1, or HNF-1
either alone or in combination. Promoter activity was examined 24 h after transfection. Expression vectors for HNF-1
(pBJ5-HNF-1
) and HNF-1
(pBJ5-HNF-1
) were gifts from Dr. G. R. Crabtree, Stanford University. The expression vector for mouse cdx-2 (pCB-mcdx-2) and its control empty vector (pCB6) were previously described (36). The sucrase-isomaltase promoter-luciferase reporter gene vector (pGL3-SI256) was provided by Dr. J. T. Troelsen (University of Copenhagen, Copenhagen, Denmark).
Reporter gene plasmid construction. A 5.4-kb fragment of the human calbindin D9k promoter (4478 to +889 bp) was obtained by PCR using human genomic DNA as template and the PCR primers: forward, 5'-GCTGCTATGGTTTGAATGCATTCC-3'; reverse, 5'-TCCTCTTCAGTTCCTCAGGAGAC-3'. A gel-purified PCR fragment was subcloned into the pCR4-Blunt vector (Invitrogen, Carlsbad, CA; pCR4-CaBP5400) and resequenced (Iowa State University DNA Sequencing Facility, Ames, IA). A full-length calbindin D9k promoter-luciferase reporter gene construct was assembled in three steps. First, a 3400-bp SacI digestion fragment of pCR4-CaBP5400 (3342 to +74) was subcloned into the SacI site of pGL3-basic (Promega, Madison, WI; pGL3-CaBP3400). Second, a 3.1-kb EcoRI fragment of pCR4-CaBP5400 (4580 to 1500) was subcloned into pCR2.1 (Invitrogen, Carlsbad, CA; pCR2.1-CaBP3100). Finally, the pGL3-CaBP3400 and pCR2.1-CaBP3100 vectors were digested with KpnI and ApaI, and the fragment from pCR2.1-CaBP3100 (4478 to 2898) was ligated into the backbone from pGL3-CaBP3400 to yield pGL3-CaBP4600 (4478 to +74 bp).
A construct lacking conserved cluster I was prepared by digesting pGL3-CaBP3400 with KpnI and NsiI. The sticky ends were blunted by using Klenow Large Fragment (New England Biolabs, Beverly, MA) and then religated to create pGL3-CaBP1700 (1558 to +74 bp). A construct lacking conserved clusters I and II was prepared by digesting pGL3-CaBP3400 with KpnI and BstXI followed by blunt-end ligation of the backbone to form pGL3-CaBP500 (408 to +74 bp). A construct lacking conserved cluster II (pGL3-CaBP1&3) was prepared by deleting the 1603-bp BbvCI fragment (2153 to 550) from pGL3-CaBP4600, whereas a construct lacking three-fourths of cluster III (pGL3-CaBP1 and 2) was prepared by deleting the 631-bp MscI fragment (710 to 79) from pGL3-CaBP4600.
Point mutations in specific response elements were introduced onto the wild-type calbindin D9k promoter-luciferase reporter gene plasmid (pGL3-CaBP4600) using the QuikChanger XLSite-Directed Mutagenesis Kit (Stratagene, La Jolla, CA) following the manufacturer's directions. The oligonucleotides used to introduce mutations were: distal cdx-2, 5'-CTCTTGTGAACACACCCTGTAA(TT/GG)ATCACTTGTCTCC-3'; distal HNF-1, 5'-CACTTGTCTCCATATATT-TTTAGT(TA/GG)ATGTTTCACAAGAGTATCTATTAG-3'; proximal C/EBP, 5'-CGACTCTGAACCATGAAGC(AA/GG)CTGTCGAGATGGACC-3'; proximal cdx-2, 5'-GGTGGCGTGCCCGT(AA/GG)AGACTATAAAAGTGTCATG-3'; and proximal HNF-1, 5'-GCCTGAGTTTCAAAAACCATT(AA/GG)TAATTACCCTTA-AATggccaac-3', where the underlined section is the response element and the bracketed bases represent the wild-type sequence followed by bolded nucleotides that replaced them in the mutated version. Plasmids with mutated response elements were isolated by using the Plasmid Mini Kit (Qiagen, Valencia, CA). All plasmids were sequenced to confirm the presence of the mutation (Iowa State University DNA Sequencing Facility, Ames, IA).
EMSA Analysis of Novel HNF-1 Response Element
Single-stranded oligonucleotides were synthesized and purified by Integrated DNA Technologies (Coralville, IA). The sequences used were lactase promoter HNF-1 site, 5'-AACCCAGTTAAATATTAAGTC-3', 125 to 105 (33); calbindin D9k distal HNF-1 site, 5'-TTTAGTTAATGTTTCACAAGAGTAT-3', 3151 to 3127; and mutated calbindin D9k distal HNF-1 site, 5'-TTTAGTGGATGGTTTCACAAGAGTAT-3', 3151 to 3127 (underlined portions refer to the HNF-1 site; the bold GG in the mutated version is the site of mutation). Double-stranded probes were made by annealing equal molar amounts of two complementary oligonucleotides in annealing buffer (10 mM Tris·HCl, pH = 7.5, 1 mM EDTA, 100 mM NaCl). The annealing reaction was conducted by heating samples at 90°C for 10 min with gentle agitation and then slowly cooling to room temperature for 1 h. The double-stranded probe was labeled with 32P by end-labeling. Briefly, 3.5 pmol of the probe was incubated with 1 µl of T4 polynucleotide kinase 10x buffer (700 mM Tris·HCl, pH 7.6, 100 mM MgCl2, 50 mM DTT), 1 µl of [-32P]ATP (3,000 Ci/mmol at 10 mCi/ml, Amersham Biosciences, Piscataway, NJ), and 1 µl of T4 polynucleotide kinase (510 U/µl) in a 10 µl reaction at 37°C for 10 min. The reaction was stopped by adding 1 µl of 0.5 M EDTA. The labeled probe was diluted 10-fold with Tris-EDTA buffer (pH = 7.4) and stored at 20°C for
2 wk. Only probes with >40% labeling efficiency were used.
Nuclear extracts were isolated from 50% confluent and 5-day postconfluent TC7 cell cultures using the Nuclear Extract Kit (Active Motif, Carlsbad, CA). Protein yield was determined by the Bio-Rad protein assay. Ten micrograms of nuclear extract were preincubated for 10 min at room temperature in binding buffer (in mM): 10 Tris·HCl, pH 7.5, 5 MgCl2, 50 NaCl, 0.5 DTT, 0.5 EDTA, and 4% glycerol plus 0.025 µg/ml poly(dIdC) with or without unlabeled competitor probes or antibodies (anti-HNF-1 antibody or goat IgG, 2 mg/ml, Santa Cruz Biotechnology, Santa Cruz, CA) in 9-µl total volume. 32P-labeled probe (0.035 pmol) was then added, and the reaction was incubated at room temperature for another 20 min, at which time 1 µl of 10x gel loading buffer was added (250 mM Tris·HCl, pH 7.5, 0.2% bromophenol blue, 40% glycerol). The whole reaction was loaded onto a 6% DNA retardation gel (Invitrogen, Carlsbad, CA), and electrophoresis was conducted by using 0.5x TBE running buffer (44.5 mM Tris base, pH 8.3, 44.5 mM boric acid, 22.1 mM EDTA) at 250 V for 15 min. The gel was dried by using a GelAir gel drying system (Bio-Rad) for 1 h, and specific bands were detected by autoradiography using Kodak XOMAT film.
Analysis of Calbindin D9k Expression in HNF-1 Null Mice
HNF-1 null mice were generated by using Cre-loxP-mediated deletion of exon 1 of the HNF-1
gene. The description and characterization of these mice has been presented elsewhere (35). Eight to twelve-wk-old HNF-1
heterozygous (+/) and age-matched HNF-1
homozygous null (/) mice were used in this study (n = 6 per genotype). Mice were anesthetized with avertin (240 mg/kg), and the proximal 1 cm of small intestine adjacent to the pylorus was removed and immediately frozen on dry ice. All dissections were conducted between 1:00 and 4:00 PM to minimize variability due to circadian expression of HNF-1
(43).
The abundance of calbindin D9k mRNA in HNF-1 +/ and HNF-1
/ mice was determined by RNase protection assays (RPA) using previously established methods (31). Total RNA was isolated from mouse tissues using the RNeas kit (Qiagen), quantified by optical density at A260 nm, and checked on an agarose gel. Antisense RNA probes for mouse calbindin D9k (a cDNA for the coding region of the mouse gene in pCR2.1) and mouse
-actin (32) were linearized, transcribed with T7 RNA polymerase, labeled by using [32P]ATP (Perkin-Elmer Life Sciences) and hybridized to RNA at 68°C in 50% formamide overnight, and digested with RNase T1 (1 µg/µl), and the protected fragments were separated on 6% denaturing polyacrylamide gels and then detected by autoradiography. The bands were quantified by using a Gel Doc system for image acquisition and Quantity One (Bio-Rad) software for analysis of band density. Calbindin D9k mRNA levels were corrected for the expression of
-actin mRNA levels before analysis. These studies were conducted under protocols approved by the Animal Research at Children's Hospital Animal Care and Use Committee.
Statistical Analysis
Data are reported as the means ± SE. Studies were examined by ANOVA or t-test (HNF-1 null mouse only) using the SYSTAT statistical software package (SAS Institute, Cary, NC). Comparisons of multiple group means were performed by using Fishers protected least significant difference. Comparisons with P < 0.05 were considered significantly different.
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RESULTS |
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In the parental Caco-2 line and the two well-differentiating clones, BBe and TC7, sucrase-isomaltase and calbindin D9k mRNA levels significantly increased as the cells differentiated (Fig. 1), and the two clonal lines expressed sucrase-isomaltase mRNA at a significantly higher level at every point after confluence (Fig. 1B). None of the three cell lines expressed high levels of calbindin D9k mRNA at 2 or 4 days in culture. However, by 8 days in culture, the calbindin D9k message was higher in TC7 (1036.40 ± 43.42 arbitrary units) than either parental or BBe cells (66.43 ± 3.97 and 86.85 ± 18.60 arbitrary units, P < 0.001, Fig. 1A). This pattern was also seen at 15 days in culture (TC7 60-fold > BBe = parental). Figure 1C shows that the level of cdx-2 mRNA was similar in proliferating cells (parental = 0.29 ± 0.04, BBe = 0.49 ± 0.01, TC7 = 0.27 ± 0.02) and increased significantly in all three Caco-2 lines from 2 to 15 days in culture (parental = 0.89 ± 0.12, BBe = 1.68 ± 0.18, TC7 = 2.23 ± 0.40).
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Regulation of Calbindin D9k Expression in TC7 Cells by 1,25(OH)2 D
1,25(OH)2 D treatment caused a small (2-fold) increase in the expression of calbindin D9k mRNA in proliferating, postproliferative, and differentiated TC7 cells (data not shown). In contrast, calbindin D9k promoter activity was not influenced by 100 nM 1,25(OH)2 D treatment, although CYP24 promoter activity was increased >100-fold under the same conditions (Fig. 2B).
Identification of Conserved Sequence Clusters and Response Elements in the Human Calbindin D9k Gene Promoter
Conserved promoter regions are more likely to contain regulatory elements controlling the expression of a gene (26). In silico analysis of the human, rat, and mouse calbindin D9k promoter sequences revealed three clusters with a high degree of homology across species. In the human promoter, these were located at 3512 to 2932 (cluster I), 1452 to 682 (cluster II) and 272 to 1 (cluster III, Fig. 3A). DNase I hypersensitive sites previously identified in the rat promoter (41) occur within cluster I (HS1), between clusters II and III (HS2 and 3), and in cluster III (HS4 and 5). Table 1 lists all of the previously reported transcription factor binding sites and relates their location to the conserved clusters we identified. Only the proximal cdx-2 response element (including the TATA box), a putative Pdx-1 response element, and the C/EBP response element at 61 bp were 100% conserved across all three species. HS2, HS3 (neither of which are intestine specific) are within a segment that was deleted in mice and humans. Of the previously identified vitamin D response elements (VDREs), none were well conserved between species (e.g., VDRE3 had missing segments in mouse and rat; VDRE1 is in a nonconserved portion of the promoter and is absent in human). SIGSCAN analysis of the three clusters identified 13 putative sites that were completely conserved among all three species, including a HNF-1 site [3131 to 3120 bp, () strand, 5'-GGTTAATNATTATCA-3', other data not shown]. We also identified two 100% conserved stretches among the species in cluster II: a 19-bp sequence [on the (+) strand starting at 807 bp 5'-TTAAACCTGCTTCTGAAGC-3'] and a 16-bp sequence [on the () strand starting at 932 bp 5'-TTTTATTTCTCATTAT-3']. The 16-bp stretch (5'-TTTTATTTC-3') is similar to a cdx-2 consensus sequence (5'-TTTTTATA/GGC-3'), but no known response element consensus sequence was found in the 19-bp stretch.
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To investigate the contribution of each conserved promoter cluster to the control of calbindin D9k gene expression, we made a series of deletion constructs as illustrated in Fig. 3A. The result of studies using these deletion constructs are shown in Fig. 3B. Removal of cluster I reduced basal promoter activity (expression in 2-day cultures) by 80% and the fold change associated with differentiation (9:2 days expression ratio) by 90% (CaBP1700). Removal of cluster II significantly increased promoter activity in both 2- and 9-day cultures by 60% (CaBP1 and 3), whereas removal of three-fourths of cluster III significantly blocked basal promoter activities as well as the fold change associated with differentiation by 50% (CaBP1 and 2).
Five cis elements were examined in this study. Within cluster I, mutation of the cdx-2 site (3158 to 3152 bp, cdx-2 mut1), the HNF-1 site (3131 to 3120 bp, HNF-1 mut1), or both of the sites (Cdx-2 mut + HNF-1 mut) reduced the basal promoter activity by 75, 80, and 75%, respectively (P < 0.01), and the fold induction due to differentiation by 12, 75, and 90% (P < 0.01), respectively (Fig. 4A). In cluster III, mutation of either the proximal cdx-2 site (40 to 25 bp, Cdx-2 mut3) or the C/EBP site (183 to 174 bp) had no detectable effect on calbindin D9k promoter activity at either stage (Fig. 4B). Similar to the removal of three-fourths of cluster III (CaBP1 and 2), mutation of the proximal HNF-1 site in cluster III (98 to 86 bp, HNF-1 mut3) decreased basal promoter activity by 36% (P < 0.01), and suppressed the differentiation-associated increase by 40% (P < 0.01, Fig. 4B).
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To further characterize the novel distal HNF-1 site in cluster I, a competitive EMSA was conducted. A major complex was formed by incubating the [32P]calbindin D9k-HNF-1 probe with Caco-2 nuclear extract from either preconfluent or postconfluent cultures. Binding in 9-day extracts was greater than that seen in 2-day extracts (Fig. 5). This complex disappeared in the presence of a 30-fold molar excess of unlabeled calbindin D9k-HNF-1 probe as well as a probe for the HNF-1 site previously characterized in the lactase gene promoter (33). A 30-fold molar excess of unlabeled mutated calbindin D9k-HNF-1 probe or a nonspecific AP2 probe did not compete with the Caco-2 nuclear extract binding to the labeled calbindin D9k-HNF-1 probe (Fig. 5). The major complexes formed with the calbindin D9k-HNF-1 probe or the lactase-HNF-1 probe could be supershifted by the addition of an anti-HNF-1 antibody, but not IgG, to the binding reaction (Fig. 5).
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In proliferating TC7 cells, which naturally express both cdx-2 and HNF-1, overexpression of cdx-2 stimulated calbindin D9k promoter activity by only 2.5-fold, whereas overexpression of HNF-1
increased calbindin D9k promoter activity by 10-fold (P < 0.001, Fig. 6B). The overexpression of both cdx-2 and HNF-1
had an additive effect on promoter activity (12-fold, P < 0.001). In HeLa cells, which lack cdx-2 and HNF-1
, overexpression of either cdx-2 or HNF-1
stimulated calbindin D9k promoter activity by 5.3-fold and 3.2-fold, respectively, and the combined overexpression of cdx-2 and HNF-1
in HeLa cells had a synergetic effect on calbindin D9k promoter activity (Fig. 6A, 14.5-fold, P < 0.001 vs. control; P = 0.012 for cdx-2 and HNF-1
interaction).
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Calbindin D9k Expression in HNF-1 Null Mice
To further define the importance of our findings regarding HNF-1-mediated calbindin D9k gene expression during enterocyte differentiation, we sought to determine whether these results could be extended to an in vivo setting. Duodenal RNA from HNF-1
knockout mice were examined for calbindin D9k expression by RPA, and this was compared with the expression seen in HNF-1
+/ mice. HNF-1
+/ mice are phenotypically normal and comparable to their wild-type littermates (35). As shown for the representative samples in Fig. 7, actin-corrected calbindin D9k mRNA levels in HNF-1
/ mice (0.16 ± 0.03 arbitrary units) were 60% lower than those of the age-matched HNF-1
+/ mice (0.41 ± 0.07 arbitrary units, P < 0.05).
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DISCUSSION |
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In contrast to the lack of vitamin D-mediated gene regulation, the calbindin D9k promoter was strongly activated during TC7 cell differentiation to an enterocyte-like phenotype. This is consistent with earlier in vivo data (24, 38, 49, 53). Previous research implicated two cdx-2 response elements as the important determinants for intestinal expression of the calbindin D9k gene (9, 34). Both elements bind to cdx-2 by ESMA (1, 9, 34), and mutation of the distal element at 3500 bp almost completely eliminated expression of a 4.6-kb rat calbindin D9k promoter-CAT reporter gene construct in transgenic mice (9). In our studies, mutation of the distal cdx-2 response element reduced basal promoter activity in TC7 cells but did not have a strong effect on differentiation-associated promoter activity. This indicates that other factors are important for increased calbindin D9k gene expression during enterocyte differentiation. We took several steps to identify these factors.
First, we showed that whereas GATA 45 and Pdx-1 have been implicated in the control of other intestinal genes, they may not be critical for calbindin D9k gene regulation during enterocyte differentiation. For example, whereas a previously identified Pdx-1 site (1) was reasonably conserved across species, Pdx-1 mRNA was not detectable in either proliferating or differentiated TC7 cells (data not shown) and therefore cannot account for the dramatic upregulation of calbindin D9k mRNA levels observed during TC7 cell differentiation. However, the participation of Pdx-1 in the regulation of the calbindin D9k gene in vivo, specifically in the duodenum in which Pdx-1 is expressed, cannot be ruled out based on our experiments. We were also unable to find phylogenically conserved GATA sites in the conserved clusters of the calbindin D9k promoter using the variants of the GATA 4/5/6 consensus sequence reported by Krasinski et al. (33). Finally, we identified a HNF-1 site that was within 25 bp of the cdx-2 response element in cluster I. Our subsequent analysis focused on the distal HNF-1 and cdx-2 sites as well as a number of phylogenically conserved sites that had been previously identified within cluster III, i.e., cdx-2 (the 5' half site), C/EBP (53 to 61 bp), and HNF-1 (86 to 98 bp) response elements (34).
The major finding of our analysis is that the newly identified distal HNF-1 site is critical for the control of both basal and differentiation-associated calbindin D9k promoter activity. Whereas mutation of the distal cdx-2 site lowered only the basal promoter activity (by 80%), mutation of the distal HNF-1 site reduced differentiation-associated calbindin D9k promoter activity by 75% and accounted for >90% of the influence of cluster I on calbindin D9k gene expression. We subsequently showed that the putative HNF-1 response element binds avidly to a protein from 9-day TC7 cell nuclear extracts, that the binding is reduced in the presence of a the HNF-1 response element from the lactase gene (33), and that the specific binding to this sequence can be supershifted by an antibody against HNF-1. In addition, a proximal HNF-1 site in cluster III is also required for basal and differentiation-associated calbindin D9k gene expression in enterocytes; mutation of this site reduced promoter activity by 40% in 9-day cultures. The impact of HNF-1 site mutations we observed in TC7 cells was similar to the reduction in calbindin D9k mRNA level we observed in HNF-1
null mice (60% reduction). This confirms that HNF-1
is important for intestinal expression of calbindin D9k and demonstrates that regulation of promoter activity through the two HNF-1
sites is physiologically relevant.
Our data identifies at least two important determinants that modulate HNF-1-mediated regulation of calbindin D9k gene expression. First is the presence of cdx-2. We found that in HeLa cells with low natural expression of cdx-2 and HNF-1
, coexpression of the two transcription factors was required for maximal induction of calbindin D9k promoter activity. When our data are considered in combination with the earlier studies by Colnot et al. (9), our studies support a model whereby cdx-2 is a permissive factor necessary for basal expression of the calbindin D9k gene in enterocytes and in which HNF-1
accounts for the increased expression of this gene along the crypt-villus axis of the small intestine. The close proximity of the distal HNF-1 and cdx-2 sites (within 25 bases) suggests that the two transcription factors may directly interact to modulate calbindin D9k gene expression; [i.e., as for the lactase gene (40)]. Additional studies will be necessary to confirm these interactions as well as to assess the potential for direct communication between the proximal and distal HNF-1 response elements.
In addition to the role that cdx-2 plays, we found that HNF-1 antagonizes HNF-1
action similar to what Boudreau et al. (4) reported for sucrase-isomaltase gene regulation. Although Boudreau et al. (4) showed that the
- to
-protein ratio falls with Caco-2 cell differentiation (from
0.8 to 0.3 due to a decline in HNF-1
levels), we found that
- to
-transfection ratios >4:1 did not completely suppress calbindin D9k promoter activity (43% reduction). This suggests that the release of HNF-1
-mediated suppression alone does not account for the dramatic increase in calbindin D9k gene expression we see during TC7 cell differentiation. Because HNF-1 and cdx-2 are both abundant in proliferating Caco-2 cells (4), a more likely mechanism for their role in calbindin D9k gene regulation is that these transcription factors are activated during enterocyte differentiation. It has been well documented that posttranscriptional modification (e.g., phosphorylation) can alter the DNA binding activity of transcription factors including cdx-2 (27, 44). Hence, it is possible that differentiation-associated changes in the phosphorylation status of HNF-1
or cdx-2 induces direct and indirect interactions between the transcription factors at critical DNA response elements or with essential coactivators (e.g., dimerization cofactor of HNF-1, cAMP response element binding protein, and CREB-binding protein-associated factors) (3, 39, 40, 48, 52). Future studies are necessary to define whether posttranslational modifications of HNF-1
or cdx-2 are necessary for differentiation-induced calbindin D9k gene activation.
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ACKNOWLEDGMENTS |
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These data were presented, in part, at the Digestive Disease Week 2002 meeting of the American Gastroenterological Association in San Francisco, CA, May 1922, 2002.
Present address of L. Wang: Center for Human Genetics, Duke University Medical Center, 4th Floor, 595 LaSalle St., Box 2903, Durham, NC.
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FOOTNOTES |
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The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
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REFERENCES |
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