(Received for publication, February 13, 1997)
From the Department of Physiology, McGill University, Montréal, Québec H3G 1Y6, Canada
The 90-kDa heat shock protein (hsp90) has been implicated in modulating steroid receptor function in vitro and in vivo. Previous studies have suggested that hsp90 interacts with large portions of the estrogen receptor (ER) ligand-binding domain and sequences of the receptor required for stable DNA binding. To characterize the interaction of the ER ligand-binding domain with hsp90, we have compared the properties of chimeras created by coupling the ligand-binding domain to the constitutive transactivator VP16-GAL. Two types of chimeras were created: VP16-GAL-ERG, containing the wild-type ligand-binding domain derived from the cDNA HEG0, and VP16-GAL-ERV, containing the substitution G400V derived from the ligand-binding domain of the original ER cDNA isolate, HE0. The G400V mutation alters the physical properties of VP16-GAL-ERV by rendering it hormone-dependent for DNA binding and more strongly dependent on estradiol for transactivation compared with VP16-GAL-ERG. Glycerol gradient analyses and chemical cross-linking/coimmunoprecipitation showed that, unlike VP16-GAL-ERG, VP16-GAL-ERV formed stable complexes with hsp90 in vitro. These data show that hsp90 selectively recognizes the altered ER ligand-binding domain containing the G400V substitution and indicate that the wild-type ER ligand-binding domain of VP16-GAL-ERG does not interact with hsp90 in vitro. Hormone binding studies showed that the ligand-binding domain of VP16-GAL-ERV was destabilized by incubation in the presence of high concentrations of salt or in the absence of sodium molybdate, conditions that disrupt its interaction with hsp90. The ligand-binding domain of the Val-400 ER thus behaves similarly to that of the wild-type glucocorticoid receptor, which has previously been shown to interact with hsp90 in vitro. These results provide evidence for the action of hsp90 as a molecular chaperone by selectively recognizing destabilized proteins.
In the absence of hormone, the estrogen receptor (ER),1 similar to all steroid receptors, has been shown to form heteromeric complexes with accessory proteins both in vivo and in vitro (1-10). Among these accessory proteins are at least two members of the heat shock protein (hsp) family, hsp90 and hsp70, as well as members of the immunophilin family and several other receptor-associated proteins. It is thought that ligand-free steroid receptors interact directly with hsp90, stabilizing the receptor in an inactive state.
The ER is a member of a large family of nuclear receptors and, as such,
is a hormone-dependent transcriptional regulator. The ER
has been subdivided into six functionally distinct domains on the basis
of sequence homology between receptors from different species (see Fig.
1) (11, 12). The highly conserved DNA-binding domain, encoded by region
C, is composed of two zinc finger motifs, each with four conserved
cysteine residues (13, 14). In addition to amino acids controlling
site-specific DNA binding, region C contains a dimerization interface
(15). Region D contains amino acids required for stable DNA binding
(16) and has been shown to stabilize interactions with accessory
proteins (1). Region E is also well conserved and contains domains
required for ligand binding as well as the ligand-dependent
transcriptional activation function known as AF-2 (17-20). Region E
also contains sequences responsible for the interaction between the ER
and accessory proteins (1, 2, 21, 22) as well as a strong dimerization
interface (23, 24). An additional transactivation function (AF-1) is provided by the poorly conserved N-terminal A/B region of the receptor,
which functions in a tissue- and promoter-specific context (18,
25).
It has been suggested that ligand binding induces a conformational change in the ER ligand-binding domain that releases hsp90, exposing those regions on steroid receptors required for homodimerization, nuclear localization, and DNA binding. Thus, hsp90 is thought to play a regulatory role by controlling several of the ligand-inducible functions of receptors. Studies in Saccharomyces cerevisiae showed that disruption of the interaction between hsp90 and the glucocorticoid receptor (GR) severely reduced the function of the GR in vivo (26, 27). Reduced expression of hsp90 strongly inhibits GR-dependent transactivation, suggesting that the GR can function properly only in the presence of hsp90. In parallel studies, however, ER-driven transactivation was less dependent on hsp90 expression, suggesting that hsp90 may be less important for controlling hormone-dependent function of the receptor in vivo.
Analysis of hsp90-ER interactions has been complicated by the overlap in domains D and E between regions of the receptor required for DNA binding, homodimerization, and nuclear localization and those required for interaction with hsp90 (1). To circumvent this problem, we recently constructed a series of chimeric ERs in which the DNA-binding domain has been replaced with that of the yeast transactivator GAL4. In addition, transactivation potential was increased by replacing the N-terminal AF-1 region with the strong acidic activator VP16, derived from herpes simplex virus, creating VP16-GAL-ER chimeras. These chimeras do not interact stably with hsp90 in vitro, bind DNA in a ligand-independent manner, and yet remain hormone-dependent for transactivation (28).
The original cDNA for the ER (HE0) contains the substitution G400V (29), which was subsequently found to destabilize the structure of the ligand-binding domain (29, 30). This suggests that the ligand-binding domain of HE0 may be like that of the hormone-free GR, which has been shown to be unstable in the absence of hsp90 (27). It was therefore of interest to determine the effect of such a destabilizing mutation on the interaction of the ER ligand-binding domain with hsp90 using VP16-GAL-ER chimeras as a model. To this end, VP16-GAL-ERV was constructed, containing the mutation equivalent to the G400V substitution of HE0. Unlike its wild-type counterpart, VP16-GAL-ERV interacts stably with hsp90 in vitro. The mutation destabilizes the ligand-binding domain, affecting its DNA binding and transactivation properties.
All chimeras were constructed in the pSG5 expression vector (31) by polymerase chain reaction amplification of the appropriate regions of VP16 and GAL4 and either wild-type ER HEG0 or HE0. Duplicates of each recombinant were tested for transactivation and verified by DNA sequencing.
Cell CultureCOS-7 cells were grown in 3.5-cm dishes in
phenol red-free Dulbecco's modified Eagle's medium (Life
Technologies, Inc.) containing 5-10% charcoal-stripped fetal bovine
serum. Lipofections were performed according to the manufacturer's
instructions (Life Technologies, Inc.). For luciferase assays, 100 ng
of receptor expression vector was transfected along with 500 ng of
17M5-TATA-Luc or ERE3-TATA-Luc reporter vector and 1 µg of
p610AZ--galactosidase expression vector for standardization. 16 h after lipofection, the medium supplemented with 10%
charcoal-stripped fetal bovine serum was changed, and cells were
incubated in the presence of 25 nM estradiol or ethanol
vehicle for a further 20 h. Cells were lysed in 250 µl of lysis
buffer (Promega). 50- and 45-µl aliquots of crude cell extracts were
used for
-galactosidase and luciferase assays, respectively. For
Western and gel retardation analyses, 1.0 µg of ER expression vector
was transfected by lipofection along with 1.0 µg of
p610AZ-
-galactosidase expression vector as an internal control. For
glycerol gradients, 10 µg of ER expression vector was transfected
into COS-7 cells plated in 10-cm dishes.
Gradients were performed essentially as described (10). Briefly, cells from six individual 10-cm plates were scraped into 6 ml of ice-cold phosphate-buffered saline containing PMSF and protease inhibitors and resuspended in 1.5 volumes of TEGM buffer (20 mM Tris (pH 7.5), 1 mM EDTA, 10% (v/v) glycerol, 30 mM sodium molybdate, and 5 mM DTT). Cells were lysed by drawing 30 times through a 25-gauge needle, and lysates were clarified by centrifugation at 12,000 rpm for 20 min at 4 °C. [3H]Estradiol (Amersham Corp.) was added to a final concentration of 25 nM, and extracts were incubated for 2 h on ice. Excess [3H]estradiol was stripped away by incubation with 0.5% activated charcoal (Aldrich) and 0.05% dextran T-70 (Amersham Corp.) for 20 min on ice. Aliquots were divided in half and adjusted to 400 mM KCl where required. Samples were loaded into 10-35% glycerol gradients in TEGM buffer in the presence or absence of 400 mM KCl along with horseradish peroxidase and glucose oxidase as sedimentation markers and centrifuged in an SW 55Ti rotor at 49,000 rpm for 16 h at 4 °C. Samples were collected in 150-µl aliquots, and 50 µl was assayed by scintillation counting. 75-µl samples were run on SDS-polyacrylamide gels to detect the fractional localization of horseradish peroxidase and glucose oxidase.
Protein Cross-linking and CoimmunoprecipitationCOS-7 cells were transfected in 10-cm plates as described above and harvested in ice-cold phosphate-buffered saline in the presence of PMSF. Cells were pelleted by centrifugation at 2500 rpm for 10 min at 4 °C. The cell pellet was resuspended in 1.5 volumes of 20 mM HEPES, 1 mM EDTA, 10% (v/v) glycerol, and 30 mM sodium molybdate in the presence of PMSF, leupeptin, aprotinin, and pepstatin. Cells were lysed by drawing 25-30 times through a 25-gauge needle, and lysates were clarified by centrifugation at 10,000 rpm for 10 min at 4 °C. Extracts were incubated in the presence or absence of 400 mM KCl on ice for 30 min. Proteins were cross-linked by incubation with 0.1 mM N-succinimidyl 3-(2-pyridyldithio)propionate (SPDP; PDI) for 30 min at room temperature. Excess SPDP was removed by running the extracts through a Sephadex G-50 spin column equilibrated in sodium phosphate buffer (pH 7.4). Samples were treated with 0.5 mM N-ethylmaleimide (10 min at 23 °C) to block all free SH groups that could prematurely cleave cross-links and divided into two equal aliquots. Intermolecular disulfide bonds formed during cross-linking were either reduced by incubation with 50 mM DTT for 30 min on ice or left intact. Protein complexes were immunoprecipitated by incubation for 12 h with a mixture of the anti-GAL4 DNA-binding domain monoclonal antibodies 2GV3 and 3GV2 on ice and then for 2 h with protein G-Sepharose (Pharmacia Biotech AG) in radioimmune precipitation assay buffer (50 mM Tris (pH 7.4), 4 mM EDTA, 150 mM NaCl, 1% Triton X-100, and 0.1% SDS). Samples were sedimented by centrifugation at 10,000 rpm for 30 s, washed three times in radioimmune precipitation assay buffer, and then resuspended in 30 µl of SDS-polyacrylamide gel electrophoresis sample buffer supplemented with 50 mM DTT. Western analysis using the anti-hsp90 monoclonal antibody SPA 835 (Stressgen Biotech Corp.) was carried out as described below.
Hormone Binding AssaysHormone binding assays were
performed essentially as described (11). Briefly, COS-7 cells were
transfected as described for glycerol gradient experiments. Cells
(10-cm dishes) were harvested in 1 ml of phosphate-buffered saline
containing PMSF and centrifuged, and the cell pellet was resuspended
and lysed as described for glycerol gradient analysis in 100 µl of
hormone binding buffer (50 mM Tris (pH 7.5), 1.5 mM EDTA, 50 mM NaCl, 10% (v/v) glycerol, 1 mM -mercaptoethanol, and the protease inhibitors PMSF,
leupeptin, aprotinin, and pepstatin) containing 10 mM
sodium molybdate where indicated. Lysates were diluted to 200 µl in
hormone binding buffer and clarified by centrifugation. For each
binding reaction, 20-µl aliquots were diluted to 50 µl with hormone
binding buffer. For preincubations with high salt, KCl was added to a
final concentration of 400 mM. Aliquots were preincubated
at room temperature as indicated, prior to incubation on ice for 5 h in the presence of 20 nM
17
-[3H]estradiol (Amersham Corp.). To determine
nonspecific binding, 4 µM estradiol was also included.
Unbound estradiol was removed by incubation with 0.5% Norit-A charcoal
and 0.05% dextran T-70 for 10 min and then centrifuged. Radioactive
estradiol in the supernatant was determined by liquid scintillation
counting.
Cells were harvested by combining
those scraped from two or three 3-cm plates in 500 µl of ice-cold
phosphate-buffered saline. Cells were centrifuged at 2500 rpm for 10 min at 4 °C; the supernatant was carefully removed; and the pellet
was resuspended in 30 µl of high salt extraction buffer (25 mM Tris (pH 7.9), 0.3 mM DTT, 0.1 EDTA, 400 mM NaCl, and 10% (v/v) glycerol). Cells were lysed by
three cycles of freezing at 70 °C and thawing at room temperature and then centrifuged at 10,000 rpm for 10 min at 4 °C, and
supernatants were stored at
70 °C. Samples were incubated for 15 min on ice in a 10-µl final volume of 25 mM Tris-HCl (pH
8.0), 1 mM DTT, 50 mM KCl, and 20% glycerol
containing 1 µg of poly(dI·dC) and then for a further 20 min at
23 °C after the addition of 50,000-100,000 cpm (5-10 fmol) of
32P-end-labeled double-stranded oligonucleotide. Samples
were run on 5% polyacrylamide gels (20:1), which were dried prior
to autoradiography.
Immunoprecipitates were run on 7.5% polyacrylamide gels containing 0.1% SDS. Resolved proteins were transferred to nitrocellulose membrane (Hybond-C, Amersham Corp.) and probed with an anti-hsp90 monoclonal antibody (SPA 835) diluted 1:1000 in Tris-buffered saline/Tween and 1% milk powder. Aliquots of extracts expressing ER chimeras were taken before or after preincubation, resolved on 10% polyacrylamide gels containing 0.1% SDS, transferred to Hybond-C membranes, and probed with anti-GAL4 DNA-binding domain monoclonal antibodies 2GV3 and 3GV2 diluted 1:5000 in Tris-buffered saline/Tween and 1% milk powder. Blots were developed using the ECL detection system (DuPont NEN).
We have recently reported the construction of a series of VP16-GAL-ER fusion receptors to study the role of hsp90 interaction in modulating ER function (28). Addition of the ER ligand-binding domain rendered constitutively active VP16-GAL partially dependent on hormone for transactivation. The VP16-GAL-ER chimeras bind DNA equally well in the presence or absence of estradiol and are at least partially nuclear in the absence of ligand (28). More important, glycerol gradient analysis and coimmunoprecipitation studies suggested that the chimeras do not interact with hsp90 in vitro (28). Assays have thus been established to measure transactivation, DNA binding, and hsp90 association by VP16-GAL-ER chimeras. We were interested next in determining the effect on the interaction of chimeras with hsp90 of the destabilizing mutation G400V, found in the original ER cDNA, HE0 (29). A well characterized chimera was chosen to study the functional differences between the Gly-400 and Val-400 homologues, containing ER ligand-binding domain sequences from amino acid 258 (Fig. 1). VP16-GAL-ERG and VP16-GAL-ERV are used to denote chimeras derived from HEG0 and HE0, respectively (Fig. 1).
Glycerol Gradient Analysis of Extracts Expressing VP16-GAL-ERV or VP16-GAL-ERG Chimerashsp90-ER chimera interactions were first probed by
glycerol gradient analysis. Sedimentation profiles of full-length
receptors were used as positive controls. In the presence of molybdate
ions, HEG0 formed a stable complex, characteristic of its interaction with hsp90, that migrated in a glycerol gradient with a sedimentation coefficient of 8-9 S. Under high ionic strength conditions, the molybdate-stabilized complex dissociated, resulting in an
"activated" ER that migrated at 4-5 S (Fig.
2A). Conversely, VP16-GAL-ERG did
not exhibit a salt-dependent shift in its migration and
sedimented at 4-5 S under both low and high salt conditions (Fig.
2B). To test the characteristics of Val-400 mutants, we
performed identical analyses on HE0 and VP16-GAL-ERV. As
expected, HE0 was found to form molybdate-stabilized, salt-sensitive 8 S complexes in vitro (Fig. 2C). Significantly,
VP16-GAL-ERV also formed a salt-sensitive 8 S complex (Fig.
2D), suggesting that hsp90 may recognize the altered
ligand-binding domain of the chimera.
Stable Interaction of hsp90 with VP16-GAL-ERV, but Not VP16-GAL-ERG, Determined by Chemical Cross-linking/Immunoprecipitation
To verify that hsp90 is indeed
a component of the 8-9 S complex containing VP16-GAL-ERV,
a combined chemical cross-linking/coimmunoprecipitation protocol was
developed using extracts of transiently transfected COS-7 cells
expressing either VP16-GAL-ERV or VP16-GAL-ERG.
Cells were lysed in the presence of molybdate ions under conditions in
which an 8-9 S complex formed in the absence of salt. Extracts were
divided into two equal aliquots; one was treated with KCl at a final
concentration of 400 mM, and the other with water alone. Cellular proteins were cross-linked using the heterobifunctional cross-linker SPDP (see "Materials and Methods"). Following
cross-linking, reactions were once more divided into two equal
aliquots, and one was treated with 50 mM DTT to reduce the
intermolecular bonds formed by SPDP. All reactions were
immunoprecipitated overnight with an antibody directed against the GAL4
DNA-binding domain. Following immunoprecipitation, proteins were
resolved on SDS-polyacrylamide gels, transferred to nitrocellulose
membranes, and probed with monoclonal antibody SPA 835 (raised against
hsp90). A 90-kDa protein recognized by SPA 835 was precipitated along
with VP16-GAL-ERV (Fig. 3, lane
1). Treatment of the extracts with DTT prior to immunoprecipitation to reduce the intermolecular cross-linker strongly
decreased the amount of detectable hsp90 that coprecipitated with the
chimera, indicating that hsp90 is not being precipitated nonspecifically by the anti-GAL4 polyclonal antibody (Fig. 3, lane 2). In the presence of 400 mM KCl, very low
amounts of hsp90 can be seen to be associated with
VP16-GAL-ERV, and this faint band disappeared upon
treatment with DTT (Fig. 3, lanes 3 and 4). This
suggests that, in the presence of KCl, only a minute amount of hsp90
may remain associated with the receptor and is consistent with the
migration of VP16-GAL-ERV at 4-5 S in glycerol gradients
under these conditions (Fig. 2).
While glycerol gradient analyses suggested that VP16-GAL-ERG does not interact stably with hsp90, we cannot rule out the possibility that hsp90 may interact transiently with the chimera in extracts. Chemical cross-linking and coimmunoprecipitation of extracts expressing VP16-GAL-ERG were therefore performed to trap any transient binding to hsp90. Even under these conditions, no coimmunoprecipitation of hsp90 was detected from extracts incubated in the presence or absence of salt (Fig. 3, lanes 5-8). Taken together, these results indicate that hsp90 selectively recognizes ER chimeras containing the G400V substitution under low salt conditions in the presence of molybdate.
The ER Ligand-binding Domain Containing the G400V Substitution Is Destabilized by High Salt and the Absence of Sodium MolybdatePrevious studies have suggested that the G400V
substitution destabilizes the ER ligand-binding domain (29). It was
therefore of interest to examine the effect of salt and molybdate ions, which modulate the stability of the interaction of the ER with hsp90,
on the stability of the G400V ligand-binding domain. Extracts of COS-7
cells transiently expressing either VP16-GAL-ERG or
VP16-GAL-ERV were preincubated for varying times in the
presence of molybdate under low or high salt conditions prior to
performing hormone binding assays. The results (Fig.
4A) indicate that high salt concentrations
only slightly affected the stability of the wild-type ligand-binding
domain of VP16-GAL-ERG. The VP16-GAL-ERV
ligand-binding domain was less stable than that of
VP16-GAL-ERG under low salt conditions and was
significantly destabilized by high salt concentrations. In addition,
the removal of molybdate from the preincubation destabilized the
VP16-GAL-ERV ligand-binding domain under low salt
conditions (Fig. 4B). A control Western analysis showed that
the loss of hormone binding activity in extracts containing
VP16-GAL-ERV was not due to proteolytic degradation of the
chimera during preincubation (Fig. 4C). These results
indicate that the VP16-GAL-ERV ligand-binding domain is
most stable at low salt concentrations and in the presence of
molybdate, conditions under which it interacts most stably with
hsp90.
Altered DNA Binding and Transactivation Properties of VP16-GAL-ERV
The effect of the G400V substitution on
the function of VP16-GAL-ER chimeras was analyzed by gel retardation
analyses performed with cognate ERE sequences in the presence or
absence of estradiol. No specific retarded complexes were formed by
high salt extracts of COS-7 cells transiently transfected with the
parental expression vector pSG5 (Fig. 5A,
lanes 1 and 2). As expected, HEG0 bound a
synthetic ERE oligonucleotide in the absence of estradiol, and addition
of hormone did not affect the level of DNA binding by the receptor
(Fig. 5A, lanes 3 and 4). In contrast,
DNA binding by HE0, which contains the G400V mutation, exhibited a
clear requirement for estradiol (Fig. 5A, lanes 5 and 6).
VP16-GAL-ERG, like HEG0, binds to cognate DNA sequences both in the presence and absence of estradiol (Fig. 5B, compare lanes 1 and 2). In this respect, it is indistinguishable from the constitutive activator VP16-GAL (Fig. 5B, lanes 7 and 8). In contrast, significant DNA binding by VP16-GAL-ERV was observed only in the presence of estradiol (Fig. 5B, lanes 5 and 6). These results show that the chimeric ERs display DNA binding characteristics that are very similar to those of their respective full-length receptors and that the G400V mutation disrupts DNA binding in the absence of hormone by both the full-length ER HE0 and the corresponding chimera VP16-GAL-ERV.
In the presence of HEG0, low but consistent levels of transactivation
of an ERE-containing reporter gene were observed in the absence of
estradiol. Hormone induced transactivation by 10-fold (Fig.
6, A and B). In contrast, no
hormone-independent transactivation over background levels was observed
in the presence of HE0, consistent with previous reports (29, 30).
Transactivation by HE0 was induced at least 20-fold by hormone.
VP16-GAL-ERG activated a 17-mer-containing reporter gene in
the absence of ligand to levels 20-30% of those seen in the presence
of estradiol (Fig. 6C). In contrast, only very low levels of
transactivation by VP16-GAL-ERV were observed in the
absence of ligand. However, in the presence of hormone,
VP16-GAL-ERV activated transcription to levels ~40% of
those seen with VP16-GAL-ERG (Fig. 6C). Thus, in
both the full-length receptor HE0 and in VP16-GAL-ERV, the
G400V substitution abolished hormone-independent transactivation (Fig.
6, B and D). Given the highly synergistic
transactivation potential of VP16 derivatives when bound to multiple
DNA elements and the observations above of
hormone-dependent DNA binding, these data suggest that
VP16-GAL-ERV does not bind to DNA at significant levels
in vivo in the absence of ligand. Western blot analysis
using a combination of monoclonal antibodies raised against the GAL4
DNA-binding domain indicated that the differences in transactivating
capabilities in the presence or absence of hormone are not due to
differing levels of protein expression (Ref. 28 and data not
shown).
Introduction of the G400V mutation into the ER ligand-binding
domain profoundly affected its interaction with hsp90. Unlike VP16-GAL-ERG, the VP16-GAL-ERV chimera formed
salt-sensitive 8 S complexes in glycerol gradients and interacted with
hsp90 in cross-linking/coimmunoprecipitation experiments (Figs. 2 and
3). This is consistent with previous observations that hsp90 could be
coimmunoprecipitated with -galactosidase-ER ligand-binding domain
chimeras derived from HE0 (21). In this respect, the isolated
ligand-binding domain of the ER mutant behaved similarly to that of the
wild-type GR, which interacts with hsp90 in vitro (21).
The G400V substitution also significantly affected ER ligand-binding domain function. Previous results indicated that the HE0 form of the ER has a reduced affinity for ligand in vitro and that this reduction may be at least partially responsible for the observed alterations in receptor function (29). Our gene transfer experiments (28) and those of others (29, 32, 33) indicate that the wild-type ER ligand-binding domain is able to dimerize in the absence of hormone both in vitro and in vivo. The G400V mutation alters the conformation of the ER ligand-binding domain to such a degree that the full-length receptor is rendered hormone-dependent for dimerization and hence DNA binding (Fig. 5) (29, 34). Our results with chimeric receptors show that the equivalent mutation can render a heterologous DNA-binding domain, which is capable of dimerizing independently, hormone-dependent for DNA binding. This suggests that the mutated ligand-binding domain sterically hinders the function of the GAL4 dimerization function or masks the amino acids responsible for DNA recognition. The effect of the G400V mutation on the interaction with hsp90, coupled with inhibition of DNA binding in the absence of hormone, provides an explanation for the observations that both HE0 and VP16-GAL-ERV are more strongly dependent on hormone for transactivation than their wild-type counterparts. These results would be consistent with mutated receptors and their chimeric homologues being maintained more stably in a cytoplasmic complex with hsp90 than their wild-type counterparts. Moreover, any dissociated receptors would homodimerize poorly and hence not bind DNA efficiently.
The conformational change induced by the G400V mutation significantly destabilized the ER ligand-binding domain. The ligand-binding domain of VP16-GAL-ERV was somewhat less stable than that of VP16-GAL-ERG under low salt conditions (Fig. 4). In addition, the ligand-binding domain of VP16-GAL-ERV, but not that of VP16-GAL-ERG, was destabilized by the addition of high salt. Similarly, the VP16-GAL-ERV ligand-binding domain was significantly less stable in the absence of sodium molybdate than in its presence. The presence of sodium molybdate and the absence of high salt are two conditions that stabilize the interaction of steroid receptors with hsp90 (1, 35). These results establish a strong correlation between the interaction of VP16-GAL-ERV with hsp90 and the stabilization of its ligand-binding domain.
The interaction of hsp90 with VP16-GAL-ERV is consistent with its acting as a molecular chaperone by binding to the destabilized ER ligand-binding domain. These results are important because hsp90 has only recently been recognized as a molecular chaperone (36, 37). They would support a model in which hsp90 selectively recognizes partially folded or partially denatured protein domains. Interestingly, hsp90 has recently been shown to stabilize the structure of the GR ligand-binding domain (27). Experiments using temperature-sensitive point mutations in the S. cerevisiae hsp90 homologue (HSP82) showed that hsp90 is required for the GR to attain a functional, ligand-inducible state. Furthermore, to remain in such a state, continuous interaction of the GR with hsp90 is required (27). The apparent instability of the GR ligand-binding domain further emphasizes its similarity to that of the HE0 form of the ER.
It is noteworthy that the ER ligand-binding domain has been used to confer hormone-dependent function on the nuclear protein Fos (38) and the cytoplasmic kinase Raf-1 (39). In both cases, the ER ligand-binding domain was derived from HE0. Based on our results, one can speculate that chimeras derived from HEG0 would be more nuclear in the absence of hormone than those derived from HE0, which would fundamentally affect the function of the resulting fusion proteins.
Current models of steroid receptor action suggest that aporeceptors form high molecular mass complexes with hsp90 and other proteins. These complexes are thought to keep the receptor in a stable inactive state until ligand binding frees it from hsp90. Indeed, both genetic and biochemical studies using the GR are consistent with this hypothesis (26, 27). Although cross-linking analysis suggests that the ER also forms complexes with hsp90 in vivo (35), several experiments have suggested that at least a portion of the hormone-free ER is nuclear and capable of binding DNA (32, 33, 40-43) and that hsp90 may not be essential for ER function (26). Taken together, these observations suggest that HEG0 interacts with hsp90 in vivo, but that this interaction is transient, resulting in dissociation, homodimerization, and nuclear transport of aporeceptors. Glycerol gradient and combined cross-linking/coimmunoprecipitation experiments (Figs. 2 and 3) did not provide any evidence that the wild-type ER ligand-binding domain interacts transiently or stably with hsp90. Previous results have shown that the isolated wild-type GR ligand-binding domain can interact with hsp90 in vitro (21). These results provide support for the idea that the ER binds less stably to hsp90 than the GR.
While our present and previous results (28) and those of others (26, 32, 33) suggest that hsp90 may not be essential for controlling the function of the native wild-type ER, it may be important for correct folding of the receptor. Genetic studies in yeast showed that reduced hsp90 levels compromised ER function, although not to the same degree as GR function. hsp90 may therefore be necessary to reduce the levels of partially folded or misfolded ER, which, once correctly folded, dissociates from the chaperone and translocates to the nucleus.
We are grateful to Drs. P. Chambon, M. Featherstone, and R. Kothary for the gifts of ER cDNAs and 17M5-TATA-Luc and p610AZ recombinants, respectively; and Drs. P. Chambon and Y. Lutz for anti-GAL antibodies.