(Received for publication, June 7, 1995; and in revised form, August 9, 1995)
From the
Treatment of HepG2 cells with known effectors of low density lipoprotein receptor (LDLR) gene expression altered the in vivo pattern of protein-DNA interactions in the promoter. The observed changes are consistent with proteins binding in vivo to the sterol regulatory element (SRE), to Sp1-like sites, as well as to other regions. Protein bound to the SRE in all conditions, but the nature of the dimethyl sulfate reactivity changed depending on the physiological state of the cell. Hypermethylation within the SRE of the low density lipoprotein receptor promoter was observed when cells were treated with cholesterol synthesis inhibitors, insulin, or phorbol 12-myristate 13-acetate, suggesting that the SRE regulates this promoter through sterol-independent as well as sterol-dependent mechanisms. No significant changes were observed in binding to the Sp1-like sites, suggesting that differential binding to these sites does not play a role in altered transcription levels. Analysis of the 3-hydroxy-3-methylglutaryl coenzyme A reductase promoter also revealed protections that varied in a cell type-specific manner. Binding to the 3-hydroxy-3-methylglutaryl coenzyme A reductase SRE and putative nuclear factor 1 sites could be observed but varied little in different physiological conditions.
The low density lipoprotein receptor (LDLR) ()and the
3-hydroxy-3-methylglutaryl coenzyme A reductase (HMGR) proteins are
responsible for regulating intracellular cholesterol homeostasis via
extracellular uptake and biosynthesis (for review, see (1) ).
The expression of these genes is highly regulated in order to provide
the cell with sufficient cholesterol for normal growth and function.
Because of the importance of these genes for a variety of cellular
processes, both are subject to regulation by multiple signals. LDLR
expression is primarily controlled transcriptionally(2) , while
HMGR expression is controlled transcriptionally, translationally, and
post-translationally(3, 4) . Effectors of LDLR and
HMGR transcription include a variety of mitogenic and nonmitogenic
signals including phorbol esters(5) , insulin(6) ,
oncostatin M(7) , transforming growth factor
,
interleukin-1
(8) , tumor necrosis factor(9) , and
platelet-derived growth factor(10) . In addition, there are a
variety of sterols that act as feedback regulators of transcription.
The manner in which this complex array of signals is integrated has not
been elucidated.
Work on localization of the DNA elements responsible for regulation of the LDLR and HMGR genes has focused primarily on the role of sterols. There is a conserved octanucleotide sequence in these promoters as well as in other cholesterol regulated genes that has been termed the sterol regulatory element (SRE)(11, 12) . However, single nucleotide mutagenesis has revealed functional differences between the LDLR and HMGR sequences, suggesting that only part of the conserved octanucleotide is functional in the HMGR promoter and that additional sequences upstream are important(13, 14) . Two related proteins, SREBP-1 and SREBP-2, bind specifically to the LDLR SRE and have been shown to be critically involved in sterol regulation(15, 16, 17, 18, 19) .
In addition to the SRE, other DNA elements corresponding to protein binding sites have been identified in both promoters. The binding of multiple factors to these promoters has been shown via in vitro DNase protection experiments and transfections using mutated promoters(2, 14, 20, 21, 22, 23) . In the HMGR promoter, a number of nuclear factor 1-like sites have been characterized by DNaseI protection while Sp1-like sites have been found flanking the SRE in the LDLR promoter (20, 24) . The importance of the Sp1 consensus site is highlighted by the deleterious effects of a single base mutation that causes familial hypercholesterolemia(25) . The sequence and previously characterized regulatory elements in the two promoter regions (26, 27) are indicated (Fig. 1).
Figure 1: Promoter sequence. The sequence of the LDLR (27) and the HMGR (26) promoters is shown for the regions that we were able to resolve. The revised numbering for the LDLR promoter is used(12) . The sequence of this region in HepG2 cells has been corrected by insertion of one A residue at -127. Sp1 and nuclear factor 1 binding sites characterized by in vitro footprinting are boxed and consensus SREs are underlined. A 9 of 11 match to the insulin response element in the phosphoenolpyruvate carboxykinase promoter (34) is marked by asterisks.
The in vitro DNaseI protection data have yielded valuable insight into regulation of these genes, but these experiments suffer from nonphysiological protein and DNA concentrations, making in vivo relevance uncertain. To directly address these concerns, we have examined protein-DNA interactions in known regulatory regions of the LDLR and HMGR promoters in Jurkat T cells and HepG2 cells. These experiments, coupled with those reported earlier in human fibroblasts and hepatocytes(28) , provide insight into the regulation of cholesterol homeostasis in a variety of cell systems. By examining alterations in the DMS-induced DNA cleavage pattern(29) , we are able to confirm and extend a number of in vitro observations as well as provide data regarding the effect of various physiological conditions on protein binding in the LDLR and HMGR promoters.
HepG2 and Jurkat T cells (both obtained from the ATCC) were
grown at 37 °C in 5% CO. HepG2 cells were grown in DMEM
medium (Life Technologies, Inc.) with 10% fetal calf serum (Hyclone)
and Jurkat cells in RPMI 1640 medium with 10% fetal calf serum
(Hyclone). DMS treatment and polymerase chain reaction conditions for
the LDLR promoter have been described previously(28) . Cells
were treated with 0.5% DMS for 1 min, spun down, and washed with cold
phosphate-buffered saline. DNA was prepared as described previously (29) and then denatured at 90 °C for 10 min in 200 µl
of 20 mM KPO
, 1 mM EDTA, chilled on ice,
and cleaved by adding 2 µl of 10 M NaOH and heating for 5
min at 90 °C. The cleaved DNA was extended with Sequenase and a
primer homologous to -255 to -240 in the LDLR promoter or
+2 to -12 in the HMGR promoter. A double-stranded oligo was
ligated to the extended DNA as described previously (29) and
amplified with one of the ligation oligos and a primer complementary to
-187 to -167 in LDLR or -14 to -33 in HMGR.
Amplification was done for 25 cycles (1 min at 94 °C, 2 min at 66
°C, 3 min at 76 °C) with native Taq polymerase, 10
mM Tris-Cl (pH 8.35), 50 mM KCl, 1.2 mM
MgCl
, and 0.2 mM dNTPs, and the mixture was
overlaid with mineral oil. Labeling of the mix was accomplished by
adding 5` end-labeled oligo (homologous to -185 to -155 for
LDLR and to -17 to -46 for HMGR), fresh polymerase, dNTPs,
and buffers, and treating for 2 min at 94 °C, 2 min at 70 °C,
10 min at 76 °C. After ethanol precipitation, the samples were
electrophoresed on a 6% acrylamide, 7 M urea gel.
mRNA levels were determined using internally controlled reverse transcriptase polymerase chain reaction reactions. Primers specific for a given gene were used to amplify both cDNA and genomic DNA and were chosen so that a small intron would allow differentiation of the cDNA and genomic DNA on a polyacrylamide gel. Since the same primers are used to amplify both the cDNA and control genomic DNA, artifacts are minimized. LDLR primers were chosen in exons 13 and 14 to flank a 134-bp intron, generating fragments of 205 and 339 bp. For HMGR, primers were designed to flank short introns based on the hamster genomic structure. Primers homologous to 2614-2637 and 2881-2858 were found to generate appropriately sized fragments, 267 bp for the cDNA and about 390 bp for the genomic DNA. For each gene, one of the primers was labeled and used to amplify each gene for 25 cycles according to conditions provided by Perkin Elmer. Samples were electrophoresed on a 5% polyacrylamide gel and quantitated using a Fuji PhosphorImager. The ratio of cDNA to genomic DNA was measured for each gene. This method of quantitation has been found to give results similar to Northerns but with less variability (data not shown).
Close contacts between protein and DNA can be identified by using DMS to alkylate the N-7 of guanine or, at a slower rate, the N-3 of adenine. Proteins bound to DNA at or near these atoms in the major and minor grooves affect the DMS reactivity at these sites. Because DMS can penetrate the cell nucleus, information about protein binding in living cells can be obtained. Previously described conditions (29) were used as a starting point for the promoter sequences of interest. Conditions were chosen so that the correct sequence was readable from DNA treated with DMS in the absence of protein, and a low background for DNA not treated with DMS was obtained. The cleavage pattern obtained with DNA isolated from DMS-treated cells was compared with the cleavage pattern from DMS-treated, naked DNA. Differences in band intensity (either protection or hyperreactivity) are caused by protein-DNA interactions. The identity of the proteins binding in vivo can then be inferred from in vitro protection experiments with purified proteins or extracts.
Because of the pivotal role of the liver in maintaining cholesterol homeostasis, we chose the human hepatoma cell line, HepG2, as a model for our protein binding studies. To distinguish tissue-specific effects, we have also examined an unrelated cell line, Jurkat T cells, for its basal response.
Figure 2: In vivo footprinting of Jurkat cells. DNA was cleaved with DMS and run on sequencing gels to determine patterns of protein binding. Regions characterized previously as protein binding sites are bracketed. The LDLR promoter is present in lanes 1 and 2 and the HMGR promoter is present in lanes 3 and 4. Lanes 1 and 3 contain DMS-treated, protein-free DNA and lanes 2 and 4 contain DNA treated with while cells were growing in RPMI plus 10% calf serum.
Detailed information about the TATA box region cannot be obtained because its AT richness provides few cleavage sites. Some protein binding can be detected, however, with protection at -27 frequently observed. In the transcriptional start region, there is hyperreactivity at -5 and protection at +2 and +3. Distal to the SRE, positions -107, -109, -110, -113, and -116 are also protected even though no binding was observed at these positions in vitro, suggestive of proteins present in vivo that are not present in the nuclear extracts or cannot bind properly in that artificial environment. Weak protection of nucleotides -131, -138, -139, -140, and -146 was also observed (data not shown), consistent with the in vitro data.
When
the HMGR promoter is examined under the same conditions (Fig. 2, lanes 3 and 4), many regions of protection and
hypermethylation are observed. In the SRE, positions -168 and
-173 are protected, while -172 shows hyperreactivity. In
the hamster HMGR promoter, three nuclear factor 1 binding sites (24) have been identified in the region we have characterized
by in vivo footprinting. In the hamster promoter, one of these
sites is a perfect match to the consensus
TGGNCCA(30) , while the other footprints were
proposed to be half-sites involved in heterodimeric
binding(24) . In the human promoter, there are four TGG
half-sites, but none of the sequences match the complete consensus
perfectly. All four of these half sites (-217 to -215,
-195 to -193, -184 to -182, and -174 to
-172) share the same modification pattern with the upstream G
protected and the downstream G hyperreactive. These four sequences are
each separated by a helical turn, suggesting that the bound proteins
are on the same face of the helix. The two downstream half-sites match
the regions shown to be important in sterol regulation in the hamster
gene. Additional sites of protection are located throughout the
promoter with especially strong sites at positions -113,
-129, -133/-137/-139 (GC box), -144,
-146, -178, and -185.
Figure 3: In vivo footprinting of HepG2 cells. DNA was treated as in Fig. 2. Lanes 1-4 contain DNA amplified using the LDLR primers, and lanes 5-8 contain DNA amplified using the HMGR primers. DNA from cells not treated with DMS is shown in lanes 1 and 5. Lanes 2 and 6 contain DNA treated with DMS after stripping away proteins. Lanes 3 and 7 contain DNA treated while cells were cultured in DMEM media with serum, and lanes 4 and 8 contain DNA from cells cultured in a serum-free medium (32) .
When the cells are switched to a defined, serum-free media, changes are seen in both promoters. While most of the LDLR footprint is unaffected by the inducing conditions (Fig. 3, lane 4), an increased hyperreactivity in the SRE at -59 and -61 was observed. Increased protection was observed over many areas of the HMGR promoter in the inducing conditions (Fig. 3, lane 8). Especially prominent is the hypermethylation at position -182, which changes to protection in serum-free medium.
Figure 4: Effect of PMA on LDLR and HMGR mRNA levels. RNA was prepared from HepG2 cells treated in parallel with those in Fig. 5. A constant amount of genomic DNA was added to each sample and then polymerase chain reaction amplifications carried out for each gene as described under ``Experimental Procedures.'' Samples taken after 0, 1, 2, 6, and 24 h of PMA treatment were run in separate lanes on a polyacrylamide gel and quantitated using a PhosphorImager. With both the LDLR and HMGR genes, the upper band is the larger genomic control, while the lower band arises from the cDNA.
Figure 5: Effect of PMA on the LDLR promoter. Lane 1 contains DNA treated in the absence of protein. Lane 2 contains DNA from cells cultured in DMEM plus 10% serum, and lane 3 contains DNA from cells that were also treated with 0.2 µM PMA for 6 h.
The only change in DMS protection that could be detected throughout the region examined was at position -59 in the SRE (Fig. 5). The extent of hypermethylation was observed to vary between experiments but could be observed as early as 1 h after the addition of PMA. Since this hypermethylation occurs concomitant with the increase in mRNA levels, it would appear that the change in protein binding indicated by hypermethylation is needed for the transcriptional increase. This is similar to the observation that fibroblasts exposed to cholesterol synthesis inhibitors or oxysterols change protein binding to the LDLR promoter prior to a change in transcription(28) .
A slight increase in the HMGR mRNA levels was observed in PMA-treated HepG2 cells at 1 and 2 h with a decrease at 24 h (Fig. 4). A 2.3-fold increase in HMGR was observed previously in THP-1 cells, but no data were provided for HepG2 cells(31) . No effects on the HMGR promoter footprint pattern were observed in response to PMA (data not shown).
Figure 6: Effect of insulin on the LDLR promoter. Lane 1 contains DNA treated with DMS in the absence of protein. HepG2 cells were cultured in a defined, serum-free media for 6 h in the presence (lane 2) or absence of insulin (lane 3).
Figure 7: Effect of ketoconazole on the LDLR promoter. Lane 1 contains DNA treated in the absence of protein. Lane 2 contains DNA from cells cultured in DMEM plus 10% serum with 10 µM ketoconazole for 24 h. Lane 3 contains DNA from identical cells to which only solvent (dimethyl sulfoxide, DMSO) was added.
The genes encoding LDL receptor and HMG CoA reductase are involved not only in regulating cholesterol homeostasis but also in other processes, many of which are specific for either LDLR or HMGR. Thus, there must be some sharing of regulatory signals while still allowing for independent inputs. Major changes in protein binding to these promoters do not occur upon transcriptional induction or between cell types. The changes we do see are focused primarily on the SRE regions of both genes (data summarized in Fig. 8). Our data are consistent with previous in vitro data on the regulation of these genes. We are also able to extend previous observations and rule out certain proposed models.
Figure 8: Summary of in vivo DMS reactivity. Regions surrounding the SREs in both the LDLR (upper) and HMGR (lower) promoters are shown. Protections are denoted with filled triangles and hyperreactivity with open triangles. Note that the LDLR promoter sequence is shown 3` to 5` in order to show the reactive purines.
In all of the conditions tested, there is virtually no change in binding to the Sp1-like sites flanking the SRE in the LDLR promoter, arguing against a major regulatory role for these sites in transcription. However, these sites are important for transcription based on both in vivo and in vitro data(2, 25) . The constancy of binding that we observe suggests a structural role in assembling the appropriate protein-DNA complex needed for transcription. It seems likely that proteins bound to these sites may serve as a scaffold for the binding of other regulatory proteins rather than carry out that function themselves.
The clear in vitro demonstration that Sp1 is able to bind to the sites flanking the SRE and the similarity of these sequences to the Sp1 consensus sequence have led to the obvious conclusion that Sp1 is binding in vivo. However, the modification patterns we observe are not completely consistent with this interpretation and suggest that there may be Sp1-like proteins that are involved. When the modification patterns of the LDLR Sp1 sites are compared with 15 previously characterized Sp1 sites (including nine characterized in vivo, (36, 37, 38, 39, 40) ), differences are observed (Fig. 9). In all 15 sites, position seven is a guanine, and it is hypermethylated in all 13 non-LDLR sites. In contrast, this position is protected in the two LDLR sites. While this does not prove the presence of a novel protein, the cloning of a family of Sp1-related proteins (41, 42) makes it a distinct possibility, especially since the LDLR sites are not perfect matches with the consensus sequence.
Figure 9:
DMS
protection pattern of different Sp1 sites. The effect of protein
binding on the DMS protection pattern is shown for the two Sp1-like
sites in the LDLR promoter as well as three additional sites (I, II, VI) characterized in the human PGK-1
promoter(38) , one site from the c-jun promoter(39) , two sites from the rat transforming growth
factor promoter(37) , one from the human platelet-derived
growth factor B (PDGF B) promoter(40) , three sites in
the SV40 early promoter(36) , and three sites from a related
monkey promoter(36) . Guanines protected upon protein binding
are shown in outline, and guanines that are hypermethylated
are shown enlarged. The nine sites in the upper half of the
figure were characterized in vivo, while the six sites in the
lower half of the figure were characterized in vitro. In the
PGK promoter, only those sites that gave consistent results across cell
lines are listed.
Because of the central role that the liver plays in cholesterol homeostasis, the regulation of hepatic LDLR expression could potentially be very different than in other tissues. The basal protein binding pattern in the LDLR promoter is virtually identical in the Jurkat and HepG2 cells examined here and the primary fibroblasts and hepatocytes examined previously(28) . While the basal protein binding pattern of the LDLR promoter does not change among these cell types, the DMS protection pattern of the SRE is altered upon transcriptional induction by ketoconazole, PMA, and insulin. In each case, the major alteration is at position -59. This could be caused either by new proteins binding to this region or by existing proteins being covalently modified or interacting with new partners. The recent cloning of proteins SREBP-1 and SREBP-2 (18) will provide reagents to aid in deciphering these possibilities.
While the cultured cells are all striking in their sameness of protein binding to the LDLR promoter, primary hepatocytes differ from other cell types in that -59 is not hypermethylated upon induction(28) . This result is not readily interpreted based on the hamster SREBP expression results. While the expression of SREBP-1 and SREBP-2 is unchanged with transcription in cultured cells, the relative expression of SREBP-1 and SREBP-2 is affected by transcription in the intact liver (18) . If the primary hepatocytes mirror the intact liver, SREBP-1 and SREBP-2 would have to yield the same protection pattern when bound to the SRE. The hypermethylation of -59 in cultured cells would then be explained not by a new protein binding to the SRE but by DNA distortion caused by more long range interactions. Additional information about the expression and processing of the SREBPs will be required to help resolve these questions.
Previous work has suggested that distinct proteins bind the SREs of the LDLR and HMGR genes(13, 14) . Homologous positions in the SRE consensus sequences are differentially methylated in Jurkat cells, supporting this conclusion. In HepG2 cells, however, the same conclusion cannot be drawn because the HMGR SRE protection pattern is similar to that seen in the LDLR SRE. The DMS profiles of purified proteins may now be undertaken to clarify the in vivo binding patterns.
These data suggest that the SRE and the protein(s) that bind to it are involved in regulating many, but not all, aspects of LDLR transcription. While the in vivo interactions identified here do not answer many of the questions about how these important genes are regulated, this information can be used to help focus future in vitro binding studies to provide a clearer picture of how these genes are regulated.