D-site Binding Protein Transactivation Requires the Proline- and Acid-rich Domain and Involves the Coactivator p300*

Claudia Lamprecht and Christopher R. MuellerDagger

From the Department of Biochemistry and the Cancer Research Laboratories, Queen's University, Kingston, Ontario K7L 3N6, Canada

    ABSTRACT
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The D-site binding protein (DBP) is a member of the proline- and acid-rich (PAR) domain subfamily of basic/leucine zipper proteins and is involved in transcriptional regulation in the liver. Deletion analysis of the DBP protein was carried out in an effort to define the function of the conserved PAR domain. Internal deletions of the protein, i.e. removing portions of the PAR domain, resulted in a substantial loss in transactivation of a high affinity DBP reporter construct when assayed in Hep G2 cells. These same sequences conferred significant transactivation to GAL4 DNA binding domain fusion proteins, indicating that this region acts as part of an independent activation domain comprised of sequences in both the amino terminus and in the PAR domain of DBP. The coexpression of full-length expression constructs for both DBP and hepatic leukemia factor resulted in a dramatic increase in activation mediated by the GAL4-DBP fusion proteins, suggesting the involvement of a regulated coactivator in this process. DBP transactivation appears to be a p300-dependent process, as a 12 S E1A expression construct disrupted DBP-mediated transactivation, and a p300 expression vector, but not a CREB binding protein vector, was able to restore DBP transactivation. These results suggest that the PAR domain is required for DBP activation, which occurs through a regulated, p300-dependent process.

    INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The D-site binding protein (DBP)1 is a member of the basic/leucine zipper family (b/ZIP) and was first isolated by its ability to bind and transactivate through an element in the serum albumin promoter (1). DBP mRNA is detected in most tissues, although the protein accumulates to high levels only in the nuclei of adult liver, suggesting that it is posttranscriptionally regulated. This 43-kDa protein is also known to undergo a robust circadian rhythm, with its expression highest at approximately 8 p.m. (2). This characteristic leads to the identification of one of its most likely target genes, the cholesterol 7alpha -hydroxylase gene (C7alpha H), which can be transactivated by DBP and which also exhibits a significant diurnal regulation (3). Other genes that appear to be regulated by DBP include PEPCK (4), alcohol dehydrogenase (5), carbamyl phosphate synthetase (6), and P450 CYP2C6 (7). DBP may also be involved in the regulation of the clotting factor IX gene and recovery of the Leyden phenotype form of hemophilia B (8, 9).

In addition to the b/ZIP domain, DBP also contains a distinct region termed the proline- and acid-rich (PAR) domain, which consists of a large number (16%) of proline, glutamate, and aspartate residues. This unique region, found immediately amino-terminal to the basic domain, shares 83% identity with two other b/ZIP transcriptional regulators, thyrothropic embryonic factor (TEF) (10) and hepatic leukemia factor (HLF) (11, 12), and together they form the subfamily of PAR proteins. TEF is expressed in the rat anterior pituitary gland and is one of the key factors in transactivating the thyroid-stimulating hormone beta  promoter (10). HLF was discovered through studies of the human pre-B acute lymphoblastic leukemia bearing 17:19 chromosomal translocations where the b/ZIP domain of HLF was found fused to the E2A gene (11, 12). HLF expression has been detected in the liver, though little is known about the roles of TEF and HLF in this tissue. All three members of the PAR subfamily recognize related sequences and are able to heterodimerize (10, 13, 14). Despite the highly conserved nature of the PAR domain, no unique function has been associated with it. Mutational analysis of the TEF PAR domain identified a cluster of six basic amino acids, referred to as the "basic extension," that is thought to be important for DNA binding specificity (10).

In this study we have been able to define a role for the PAR domain of DBP in the transactivation potential of this protein. Through the use of deletion mutants within the context of the whole DBP protein, we have demonstrated that sequences within the central 28 amino acids of the PAR domain are essential for DBP to transactivate a site from the C7alpha H promoter. Using GAL4 DNA binding domain fusion proteins, we have shown that the PAR domain must act in conjunction with sequences within the amino terminus of DBP to mediate transactivation. Interestingly, cotransfection of full-length DBP or HLF was able to dramatically increase the transactivation potential of these GAL4-DBP fusion constructs. Cotransfection of an E1A vector was able to inhibit DBP-mediated transactivation. Introduction of a p300 expression vector was able to overcome the E1A-mediated inhibition. These results indicate that DBP transactivation is a p300-dependent process.

    MATERIALS AND METHODS
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nuclear Extracts and DNA Binding Assays-- Nuclear extracts were prepared from Hep G2 cells transfected by calcium phosphate coprecipitation with DBP and DBP/GAL4 expression vectors. After 48 h, three 100-mm tissue culture dishes transfected with each construct were washed, and the cells were collected and spun at 1000 × g for 5 min. The pellet was resuspended in 4 ml of lysis buffer (10 mM Hepes, pH 7.6, 100 mM KCl, 0.1 mM EDTA, 3 mM MgCl2, 10% glycerol, 1 mM dithiothreitol, 1% Trasylol, and 1 µg/ml leupeptin/pepstatin A) and ruptured with 10 strokes of a Dounce homogenizer. The mixture was spun at 500 × g for 5 min, and the pellet was resuspended in 1 ml of the above lysis buffer. Cells were again pelleted for 2 min at 15,000 × g in a microcentrifuge, and the protein was extracted by resuspension in 150 µl of lysis buffer with 0.27 M KCl. This mixture sat on ice for 15 min with intermittent mixing, was spun for 15 min at 15,000 × g, and the protein-containing supernatant was stored at -70 °C.

Gel mobility assays were performed as described previously (8). The sequences of the oligonucleotides used in these experiments are as follows. D-site   5'- TGGTATGATTTTGTAATGGGG ACTAAAACATTACCCCACCAT-5' C7alpha H   5' -CTTTGGATGTTATGTCAGCA          CCTACAATACAGTCGTAAAG-5' 17-G4M   5'-AGCTTCGGAGGACTGTCCTCCG           GCCTCCTGACAGGAGGCTTCGA-5' Oligonucleotides 1-3 for bandshift probes

Supershift experiments were carried out by the preincubation of the antibody with the protein extracts in the bandshift binding reaction for 30 min on ice, followed by the addition of the radiolabeled oligonucleotide. Rabbit antibodies raised against the full-length recombinant DBP protein were used to detect DBP among nuclear proteins and extracts in both bandshift and Western assays.

Expression and Reporter Constructs-- A DBP-responsive reporter construct was created by oligomerization of the C7alpha H oligonucleotide (see above) followed by blunting of the overhang using Klenow polymerase. Size-selected material was then cloned into the G-free/TATA/LUC construct at the SmaI site. This vector has previously been described (9) and includes the luciferase gene cloned downstream of the G-free cassette. This allows for both in vitro transcription and mammalian transfection experiments to be carried out with the same vector. A GAL4-responsive reporter construct was created using the same G-free/TATA/LUC vector and involved the recloning of the dimer GAL4 site from 17M2-G.CAT using HindIII and PstI sites upstream of the TATA box.

All full-length DBP sequences were cloned into the pSCT expression vector downstream of the cytomegalovirus promoter. The PARN construct was created by insertion of an EcoRI/BamHI fragment encoding the NH2-terminal portion of DBP (amino acids 1-185) upstream of the EcoRI/HindIII PAR-bZIP-COOH-terminal fragment (amino acids 188-325). Each PAR deletion construct contains the NH2-terminal fragment with the bZIP and COOH-terminal portions of DBP with decreasing amounts of the PAR domain (PARN, amino acids 187-253; PAR2, amino acids 207-253; PAR2.1, amino acids 214-253; PAR2.2, amino acids 226-253; PAR3, amino acids 235-253; BXT, amino acids 243-253).

GAL4 fusion constructs were made using the GAL4 DNA binding domain (amino acids 1-148) in the vector G4MpolyII. Vectors containing the PAR domain alone were cloned into XhoI/KpnI, downstream of the GAL4 DNA binding domain. Constructs, including the NH2-terminal portion of DBP upstream of the PAR domain deletions listed above, were also inserted using XhoI and KpnI.

Cell Culture and Cotransfection Experiments-- Transient transfection assays were carried out as described previously, using the calcium phosphate precipitation method into Hep G2 cells grown in Dulbecco's modified Eagle's medium (Life Technologies, Inc.) with 10% fetal bovine serum. A total of 20 µg of DNA was transfected per 100-mm plate and consisted of 5 µg of the reporter construct and 3 µg of a beta -galactosidase expression vector, pCH110 (Amersham Pharmacia Biotech). In cotransfection experiments, 2 µg of pCMV-DBP was added. Luciferase and beta -galactosidase assays were carried out according to the manufacturer's instructions (Promega). The constructs used were either the multimerized C7alpha H DBP site in the G-free/TATA/LUC construct or the GAL4 consensus sequence reporter construct. In cotransfection experiments using the GAL4 fusions, 2 µg of the-GAL4-DBP constructs were added, either alone or with 500 ng of full-length DBP (CMV 28) and 5 µg of the reporter construct 17M2-GLUC. All transfections contained 3 µg of pCH110 (Amersham Pharmacia Biotech) and expressed the beta -galactosidase gene, which acted as an internal control.

In cotransfection experiments with CBP (a gift of Dr. Richard Goodman) and p300 and E1A (a gift of Dr. David Livingston) expression vectors, 1 µg of PARN was added, either alone or in combination with 0.25 µg of E1A and differing concentrations of p300 or CBP (0.1-5 µg) and 2.5 µg of the reporter construct. All transfections contained 1.5 µg of the pCH110 control plasmid.

    RESULTS
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Deletion Analysis of the PAR Domain-- The three known members of the PAR domain family, DBP, TEF, and HLF, share a domain of high sequence identity but unknown function. To determine whether the PAR domain (amino acids 188-253) was required for DBP function, progressive internal deletions from amino acid 188 through the entire PAR domain were created (see Fig. 1 for PAR domain sequence and location of deletions). These constructs preserved the amino-terminal half of DBP as well as the b/ZIP domain so that changes in DNA binding specificity were expected to be minimal. Previous studies have demonstrated the ability of DBP to transactivate via the high affinity albumin D-site in Hep G2 cells. In this work we have taken advantage of a reporter construct consisting of multimerized DBP binding elements derived from the C7alpha H promoter (3) cloned in front of the albumin TATA box and driving a G-free cassette as well as the luciferase gene. This vector has proven to be more specific for DBP than the albumin D-site element, as transactivation due to the presence of CCAAT/enhancer binding protein alpha  in these cells is considerably reduced with this construct. Expression of the full-length DBP construct results in an over 250-fold increase in promoter activity (Fig. 1B) compared with the empty expression vector (PSCT). Deletion of the first 20 amino acids (PAR2) resulted in little change in transactivation. However, progressive deletions through the next 27 amino acids resulted in a steady loss of activity. The PAR3 construct was reduced to a 30-fold activation, whereas the BXT construct (which eliminates the PAR domain completely) was essentially inactive. These results indicate that the PAR domain is critical for DBP transactivation and that a core region of close to 30 amino acids within this region is of particular importance.


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Fig. 1.   Analysis of deletions through the DBP PAR domain. A, the amino acid sequence of the DBP protein from amino acids 188-306, comprising the PAR, basic, and part of the leucine zipper domains, is illustrated. The location of various deletions of the PAR domain are indicated by the horizontal arrows, with the name of the corresponding mutant appearing above the arrow. The sequences of the comparable regions of TEF and HLF are also shown, with regions of sequence identity with DBP being boxed. The shaded boxes indicate the location of hydrophobic residues in the leucine zipper. B, transactivation mediated by DBP bearing internal deletions of the PAR domain. Mammalian expression vectors containing DBP cDNAs with the internal deletions indicated above, were introduced into Hep G2 cells using calcium phosphate transfection, along with a luciferase reporter construct bearing repeated DBP binding elements derived from the cholesterol 7alpha -hydroxylase gene promoter. Transfection efficiencies were corrected using a beta -galactosidase expression vector (pCH1101) and are expressed as a -fold increase in activity over the reporter construct with the empty expression vector (PSCT). PARN represents the full-length DBP expression vector. The averages of three transfections are indicated (solid boxes), with the standard deviations shown by the shaded boxes. C, analysis of DBP proteins bearing internal deletions of the PAR domain. Large scale transfections of Hep G2 cells were carried out using the various DBP expression vectors, and nuclear extracts were prepared using high salt extraction. These nuclear extracts were tested for DBP DNA binding activity using a bandshift assay with the cholesterol 7alpha -hydroxylase and albumin D-sites. The names of the constructs are indicated above each lane. PSCT refers to the transfection of the empty expression vector, and MOCK refers to untransfected cell extracts. The location of DNA-protein complexes is indicated (B), as is the position of the free DNA (F).

To confirm that the decreased transactivation mediated by the PAR domain deletions was not the result of changes in protein stability or DNA binding, nuclear extracts of Hep G2 cells transfected with the various constructs were prepared. Western blot analysis indicated that all of the constructs produced comparable amounts of protein with the expected mobility (data not shown). The extracts were then normalized for equal amounts of DBP protein and were used in gel mobility shift assays, with the DBP binding elements from the C7alpha H gene promoter (-237 to -212) (3) and the D-site of the albumin promoter (1) as probes. Two different probes were used to determine whether these mutations altered binding specificity. All of the PAR deletions appear to have a slight increase in DNA binding activity compared with the wild type sequence. Little or no decrease in relative DNA binding activity was observed with either probe until a region known as the basic extension was removed (Fig. 1C, BXT), which resulted in complete loss of DNA binding activity. This is consistent with the reported involvement of this region in modulating DNA binding specificity in TEF. In contrast to the other deletion mutants, the DNA-protein complex formed with the PAR3 construct was characteristically diffuse. This change in migration may be associated with conformational changes in DBP or alterations in binding of associated proteins. Overall, these results indicate that the observed decrease in DBP-mediated transactivation upon removal of parts of the PAR domain (through to PAR3), is the result of changes in intrinsic transactivation activity and not the result of reduced DNA binding activity. Clearly, removal of the basic extension does have a dramatic effect on DNA binding, resulting in complete loss of transactivation.

Transactivation mediated by DBP has previously been shown to be tissue-specific, being active in Hep G2 cells, which are derived from a hepatocellular carcinoma but inactive in L cells (1). To determine whether the PAR domain plays a role in this tissue-specific activation, the cotransfection experiments with the PAR deletions were preformed in CV-1 cells, a monkey kidney cell line. No transactivation was observed in this cell line even with the deletions (data not shown), indicating that the PAR domain does not play a negative role in the generation of tissue specificity. As DBP only transactivates in Hep G2 cells, it is possible that other factors that are liver-specific may be required for DBP transactivation.

The PAR Domain Is Part of the Transactivation Domain-- To determine whether the PAR domain functions independently as a transactivation domain, fusion constructs with the GAL4 DNA binding domain were created. Each of the PAR deletion constructs, in conjunction with the entire NH2-terminal portion of DBP (amino acids 1-185), was fused upstream of a 147-amino acid region of GAL4, encoding its DNA binding domain in an SV40-based expression vector. The GAL4-responsive reporter construct consisted of two repeats of the GAL4 binding site cloned into the G-free/TATA/LUC reporter construct (see Fig. 3A). Transfection with a construct containing the entire amino-terminal and PAR domains of DBP into Hep G2 resulted in a 24-fold increase in activity (Fig. 2A, GNPN) compared with transfection of the GAL4 DNA binding domain alone (G4M). Progressive deletion of the PAR domain in the presence of the amino terminus resulted in a decrease in transcriptional activity similar to that seen with the whole protein (Fig. 2A: GNP2, 11-fold; GNP2.1, 11-fold; GNP2.2, 4-fold; and GNP3, 4-fold). This effect of the PAR domain was dependent on sequences within the amino terminus, as the PAR domain alone (GP, 0.9-fold) exhibits no activity.


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Fig. 2.   Transactivation and DNA binding activity mediated by GAL4 fusion proteins containing DBP amino and PAR domains. A, the DBP amino-terminal region, in conjunction with various segments of the PAR domains (as indicated in Fig. 1), was inserted downstream of the GAL4 DNA binding domain in a mammalian expression vector. GP is the PAR domain without the amino-terminal region of DBP. These constructs were then assayed for transactivation of a GAL4 reporter construct in Hep G2 cells. Transfection efficiencies were corrected using a beta -galactosidase expression vector and are expressed as a -fold increase in activity over the reporter construct with the GAL4 expression vector. The averages of three transfections are indicated (solid boxes), with the standard deviations shown by the shaded boxes. B, bandshift assays using a GAL4 recognition site were carried out with extracts prepared with the GAL4 expression constructs (left). The location of DNA/protein complexes is indicated (B), as is the position of the free DNA (F). A DBP polyclonal antibody was also added to the bandshift reaction (right, +Ab). The location of the supershifted complexes is indicated (SS), with the typical DBP complex remaining in the well. The construct containing the PAR domain alone produced a distinct supershifted complex.

To address whether the deletions alter protein stability or DNA binding activity, nuclear extracts from Hep G2 cells transfected with each of the GAL4-DBP deletion constructs were prepared. Western blot analysis using a DBP antibody indicated that all of the fusion proteins produced comparable amounts of protein (data not shown). Bandshift assays with these extracts were also carried out using the GAL4 recognition site. The complexes formed with the GAL4 fusion containing only the PAR domain (Fig. 2B, GP) or the GAL4 DNA binding domain alone (G4M) were distinct. However, the other N-terminal-containing proteins formed relatively diffuse complexes. A supershift experiment with a DBP antibody was used to specifically identify the fusion protein binding component (Fig. 2B, +Ab). All of the DBP-containing proteins produced a comparable amount of supershifted complex (SS) (slightly less GNP2.2 was added in this experiment). Overall, these results suggest that the differences in transactivation mediated by the GAL4 fusions are likely because of an intrinsic activity of these proteins rather than changes in the amount or DNA binding activity of the proteins produced.

The PAR Proteins Modulate DBP Transactivation-- Deletions of the PAR domain in the context of the GAL4 constructs produced an effect very similar to that observed with the whole protein. However, comparison of the level of transactivation obtained with the GAL4 fusions with that of the whole DBP protein or with GAL4 constructs containing the VP16 activation domain revealed that the activity of the GAL4-DBP fusion construct was relatively low. The only domain not included in the GAL4 constructs was the b/ZIP domain, which is involved in DNA binding and dimerization. This disparity in activity suggests that either dimerization was required for optimal transactivation or that the presence of a functional protein increased transactivation. The GAL4 transactivation experiments were repeated in the presence of expression vectors for full-length DBP or the related PAR protein, HLF. DBP and HLF together produced the most dramatic increase in transactivation, with over a 10-fold increase in activity (Fig. 3B). This activity was dependent on the presence of both the amino-terminal domain and the PAR domain, as constructs containing either domain alone (Fig. 3A, GPN and GNP3) exhibited little stimulation in the presence of the PAR proteins (Fig. 3B). Interestingly, CCAAT/enhancer binding protein alpha , which recognizes many of the same sites as DBP, was unable to activate the GAL4-DBP fusion construct (data not shown). The absence of the b/ZIP domain in the GAL4 fusion proteins should prevent interaction between the fusion protein and the full-length PAR proteins. Attempts to demonstrate physical interaction, either in vivo or in vitro, have failed. These results suggest that the full-length PAR proteins in some way modulate the activity of cellular components involved in transcriptional activation. The requirement of this modulated factor for optimal transactivation mediated by DBP suggests that this factor has the properties of a coactivator.


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Fig. 3.   Cotransfection of DBP and HLF augments transactivation by the GAL4-DBP fusion proteins. A, a schematic diagram of the GAL4 constructs with the amino and PAR domains (GNPN), the PAR domain alone (GPN), the amino terminus and the PAR3 deletion (GNP3), or the vector containing the GAL4 DNA binding domain alone (G4M) is shown. The reporter construct is also pictured, consisting of two repeats of the GAL4 recognition element (2X GAL4 R.E.), a TATA sequence derived from the albumin gene (ALBUMIN TATA), a G-free cassette (G-FREE), and the luciferase gene (LUCIFERASE). B, the GAL4-DBP fusion constructs were transfected into Hep G2 cells either with the reporter construct or with expression vectors for both wild type full-length DBP and HLF genes (+DBP/HLF). Transfection efficiencies were corrected using a beta -galactosidase expression vector and are expressed as a -fold increase in activity over the reporter construct with the GAL4 expression vector (G4M). The averages of three transfections are indicated (solid boxes) with the standard deviation shown by the shaded boxes.

DBP Transactivation Is a p300-dependent Process-- The adenoviral early protein E1A has been shown to inhibit specific gene expression, as well as the induction of differentiation, in several model systems by inhibiting the coactivators p300 and CBP (15). To determine whether these proteins play a role in DBP-mediated transactivation, a 12 S E1A expression vector was cotransfected along with the wild type DBP vector and the multimerized C7alpha H-site reporter construct. Binding of DBP to its response element in this experiment resulted in a 250-fold increase in activity (Fig. 4A). The coexpression of E1A reduced this activity by a factor of 10, suggesting that a protein bound and inactivated by E1A was involved in this process. To directly test whether it is p300 or CBP that is required for DBP activity, complementation of the E1A inhibition was attempted using expression vectors for both proteins. Increasing concentrations of a p300 expression vector were introduced along with the E1A-containing vector. Relatively low concentrations of the p300 expression vector were able to completely restore DBP transactivation (Fig. 4A), though this effect decreased at higher p300 levels. The effect of introducing p300 alone, without E1A, was also examined. At the highest concentration of p300 vector used, DBP-mediated transactivation was reduced to approximately 10% (Fig. 4A), the same level as observed with the E1A expression vector. The tendency of p300 to form inactive aggregates when cotransfected may sequester the endogenous p300, as has been observed previously (16), resulting in the reduced activity observed. In the presence of E1A, overall p300 levels must be stabilized, allowing for complementation. Cotransfection of an expression vector for CBP, which can also bind E1A, did not have any effect on DBP transactivation or on the inhibition of transactivation by E1A (Fig. 4B). Even though both p300 and CBP bind E1A, it is possible that p300 simply sequesters E1A, preventing it from inhibiting some other cellular factor. A p300 mutant that lacks the E1A binding domain (p300Delta 30) but is still functional (16) was used in the same complementation assay. It resulted in comparable complementation to the wild type p300 construct (Fig. 4C). Interestingly, expression of the p300Delta 30 construct alone did not inhibit transactivation. This may be the result of a reduced tendency of this p300 mutant to aggregate (16). Overall, these experiments demonstrate that DBP transactivation requires a coactivator that can be inhibited by the adenoviral E1A protein and that this coactivator is likely p300.


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Fig. 4.   p300 overcomes the E1A-mediated inhibition of DBP transactivation. A, a DBP expression vector (PARN) was cotransfected into Hep G2 cells along with the C7alpha H reporter construct. A 12 S E1A expression vector was also added in conjunction with the other plasmids (+E1A). In addition, the indicated amount (in µg) of a p300 expression vector was also included with (PARN+E1A+p300) or without (PARN+p300) the E1A vector. The -fold increase in activity in relation to the reporter and empty expression vector (PSCT) is indicated. The averages of three transfections are indicated (solid boxes) with the standard deviations shown by the shaded boxes. B, as above, except with the addition of an expression vector for CBP, with (PARN+E1A+CBP) or without (PARN+CBP) E1A. C, as above, except with the addition of an expression vector for p300Delta 30, which contains a deletion that removes the E1A binding region of p300 but otherwise maintains its activity.


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The members of the PAR domain family of proteins are unique among the b/ZIP class of factors in having an extended region of homology outside of the b/ZIP domain itself. Previous studies have implicated a relatively restricted part of the PAR domain, called the basic extension, in site-specific recognition (10). However, a role for the relatively large remaining portion of this domain has not previously been defined. We have been able to demonstrate a requirement for this domain in transactivation mediated by DBP. Deletions that remove amino-terminal parts of the PAR domain but that do not effect DNA binding activity are severely debilitated in their ability to activate transcription via a high affinity DBP binding site. These same sequences are required for activity of the GAL4 fusion proteins, and again this region functions in conjunction with other sequences present in the amino-terminal part of DBP, as either domain alone is inactive. The amino-terminal domains of all three PAR proteins have a 28-amino acid region of high similarity that may comprise the functional part of the amino-terminal region of DBP (17). It has been shown that this isolated segment from TEF acts as a transcriptional activator when assayed outside the context of the whole protein (10). We have found similar results with this amino-terminal region of DBP (data not shown). It may be that other sequences in these proteins inhibit the amino-terminal activation domain, which the PAR domain overcomes. Alternatively, the isolated amino-terminal activation domain may interact with a different part of the transcriptional machinery compared with the intact protein. The amino-terminal and PAR domains may represent separate contact points for the same protein or may contact two different proteins where both are required for function. The conserved nature of both the amino-terminal and PAR domains of all three known PAR domain proteins, coupled with their similar tissue distribution, suggests that they interact with the same protein or a closely related factor.

Transcriptional activation occurs either through the direct recruitment of parts of the transcriptional machinery such as TFIID or in conjunction with coactivators. The coactivator p300 is known to interact with a wide variety of b/ZIP factors including CREB (18), c-Jun (19), and CCAAT/enhancer binding protein beta  (20). It functions as a histone acetyltransferase (21) and may act to create a chromatin environment favorable for transcription (22). The p300 protein has been implicated in the regulation of differentiation in a variety of systems (23) and has been shown to undergo increased phosphorylation in response to differentiation (24). The ability of p300 to overcome E1A-mediated inhibition of DBP transactivation strongly suggests that this coactivator is required for the transcriptional activity of DBP. The inability of CBP to complement the E1A-mediated repression of DBP clearly differentiates the functions of p300 and CBP in this context. The dependence of DBP transactivation on a coactivator, rather than directly recruiting the transcriptional machinery, implies a requirement for regulation of this activity. This may be linked to changes in gene expression associated with terminal differentiation of the liver when DBP is exclusively expressed (1). The ability of DBP and HLF expression to increase DBP transactivation and to up-regulate the DBP promoter (25) suggests that some form of autoregulation of PAR protein activity involving p300 may occur in liver cells.

    ACKNOWLEDGEMENTS

We thank Dr. Richard Goodman, Dr. David Livingston, and Dr. Richard Eckner for supplying numerous constructs used in this study.

    FOOTNOTES

* This work was supported by funds from the National Cancer Institute of Canada through funds provided by the Canadian Cancer Society.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.

Dagger Research Scientist of the National Cancer Institute of Canada, supported by funds provided by the Canadian Cancer Society. To whom correspondence should be addressed: Cancer Research Laboratories, Botterell Hall, Queen's University, Kingston, Ontario, K7L 3N6 Canada. Tel.: 613-533-6751; Fax: 613-533-6830; E-mail: muellerc{at}post.queensu.ca.

    ABBREVIATIONS

The abbreviations used are: DBP, D-site binding protein; PAR, proline and acidic rich; b/ZIP, basic/leucine zipper; C7alpha H, cholesterol 7alpha -hydroxylase; PEPCK, phosphoenolpyruvate kinase; TEF, thyrothropic embryonic factor; HLF, hepatic leukemia factor; CREB, cyclic AMP response element binding protein; CBP, CREB binding protein.

       REFERENCES
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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