From the Department of Biochemistry and Molecular Biology, University of Miami School of Medicine, Miami, Florida 33136
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ABSTRACT |
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Mapping of tryptic phosphopeptides of heat shock factor 1 (HSF1) from non-stressed or moderately heat-stressed HeLa cells, labeled in vivo by [32P]orthophosphate, revealed four major phosphopeptides A to D. Heat stress drastically increased phosphopeptide signals. To identify target peptides and amino acids and to correlate phosphorylation and transactivation function, phosphopeptide maps were produced of LexA-human HSF1 chimeras and mutant derivatives thereof, and transactivation activities of original and mutant chimeras were compared. LexA-HSF1 chimeras were previously shown to be regulated identically to HSF1, except that they transactivate promoters with LexA-binding sites instead of hsp promoters. The patterns of phosphopeptides of LexA-HSF1 and endogenous HSF1 were similar. Analysis of single residue substitutions suggested that phosphopeptide C is peptide VKEEPPSPPQSPR (297-309) phosphorylated on Ser-307 but not Ser-303. Substitution of Ser-307 but not Ser-303 caused deregulation of factor activity. Mapping of several constitutively active chimeras associated unphosphorylated peptide C with the transcriptionally active HSF1 conformation, suggesting that dephosphorylation of this peptide (at Ser-307) may either be an integral step in the activation process or serve to maintain the active conformation of HSF1. Exploiting this correlation, indirect evidence was obtained that activation domains of HSF1 interact with the distantly located regulatory domain to maintain the factor in an inactive state.
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INTRODUCTION |
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Stress-induced expression of heat shock protein (hsp)1 genes is controlled by heat shock factor (HSF) (HSF1 in vertebrate species; Refs. 1-5)). Activation of HSF1 is generally thought to involve at least two distinct regulatory steps. In the first step, cytoplasmic, non-DNA-binding HSF1 is converted to a homotrimer that is DNA-binding. This homotrimeric factor translocates to the nucleus and binds to heat shock element (HSE) sequences of hsp promoters (6-8) but is incapable of enhancing transcription from these promoters (9-11). In a second step, the inactive HSF1 trimer is converted to the active transcription factor. Support for this sequence comes from the observation that in some circumstances (10, 12, 13), e.g. exposure to sodium salicylate (10) or menadione (12), only the first step can be triggered, and in others, e.g. overexpression from a transfected HSF1 gene (11), the first step is bypassed. Mutagenesis experiments identified elements in the 529-residue-long human HSF1 sequence, located between residues 186 and about 315 and collectively referred to herein as regulatory domain, that are involved in keeping trimeric factor in an inactive state in the absence of stress (11, 14, 15).
HSF1 is phosphorylated at serine and threonine residues in unstressed cells (16, 17). Following heat shock or when cells are exposed to one of several chemical stressors, the transcription factor becomes hyperphosphorylated (1, 4, 18). During recovery of cells from such stress, HSF1 is dephosphorylated to its pre-stress state.
Regarding the possible role of constitutive phosphorylation, Mivechi and Giaccia (19) found that overexpression of a dominant inhibitory mutant of ERK1 increases the expression of an hsp70 promoter-driven reporter gene in NIH-3T3 cells. Knauf et al. (20) have shown that expression of actived Raf in human 293T cells results in increased phosphorylation of a flag epitope-tagged HSF1 expressed from a transfected gene. Chu et al. (21) performed experiments involving co-transfection of NIH-3T3 cells with an hsp70-CAT reporter gene and with expression vectors for human HSF1 and MEK-1 and noted that overexpression of MEK-1 reduces reporter gene expression. Although their physiological relevance remains uncertain, these observations demonstrate that, under conditions of maximal activation of the MAP kinase pathway, HSF1 is phosphorylated by MAP kinase, and its activity is inhibited.
Inhibitors of Ser/Thr kinases partially inhibit heat-induced hyperphosphorylation of human HSF1 and prevent increased Hsp expression but do not affect HSF1 trimerization and HSE DNA-binding activity (17), suggesting that induced phosphorylation is required for the second but not the first step in the activation of HSF1. In agreement with these observations, HSF1 hyperphosphorylation is induced more slowly than trimerization and correlates better with the acquisition of transcriptional competence (16). A role of induced phosphorlyation in activating the transcription function of the factor is also implied by experiments involving overexpression of HSF1 in human cells from a transfected gene. The exogenous HSF1 that is trimeric but transcriptionally inert can be activated by calyculin A, an inhibitor of Ser/Thr protein phosphatases (17). Although suggestive, these data are correlative in nature, and there is no direct proof for any functional role of HSF1 hyperphosphorylation.
While most HSF1 is in a non-trimeric form in unstressed human cells, a low level of transcriptionally inert HSF1 trimers could be detected (17). If this finding reflects the continuous assembly and disassembly of HSF1 trimers, the substrate of constitutive phosphorylation may be either the non-trimeric or the trimeric factor, or both. For the purposes of this study, the question of whether non-trimeric or trimeric factor is the target of phosphorylation did not need to be resolved since similar phosphopeptide patterns were obtained from non-trimeric and trimeric endogenous HSF1. The substrate for stress-induced phosphorylation most likely is the inactive HSF1 trimer since trimerization (measured as DNA-binding activity) precedes induced phosphorylation of the factor (16). Further support is provided by findings that exposure of cells to certain chemicals or transfection with an HSF1 gene results in trimeric, under-phosphorylated and transcriptionally inert HSF1 that is hyperphosphorylated and activated by heat shock or by addition of an inhibitor of protein phosphatases (9, 17). Thus, the preferred substrate for in vivo mapping of phosphoamino acids is trimeric HSF1. In the present study, to allow for parallel assays of phosphorylation and transcription factor function, a trimeric (because expressed from transfected genes) chimeric HSF1 was used in which the HSE DNA-binding domain was substituted by the DNA-binding domain (only) of bacterial repressor LexA. This chimeric factor is known to be regulated in a fashion that is indistinguishable from wild-type HSF1, except that it binds a LexA recognition site rather than an HSE sequence (11, 22). Initial in vivo mapping experiments confirmed that the chimeric factor is also phosphorylated similarly to endogenous HSF1.
Previous studies, mapping phosphopeptides of GAL4-human HSF1 chimeras or of recombinant HSF1 phosphorylated in vitro, concluded that HSF1 is constitutively phosphorylated on residues 303 and 307, and transactivation assays suggested that phosphorylation at residue 303 plays an important role in repressing the transcriptional ability of the factor (16, 20, 21). The present study is relying on phosphopeptide mapping of a fully functional, trimeric HSF1, i.e. LexA-HSF1 chimera, and of mutant derivatives thereof labeled in vivo and on transactivation assays with the same molecules to both revisit and extend previous observations. Our experiments revealed four major, 32P-labeled, tryptic peptides of HSF1 (phosphopeptides A to D). Mapping data obtained from mutant LexA-HSF1 chimeras are consistent with the view that phosphopeptide C corresponds to peptide VKEEPPSPPQSPR (residues 297-309) phosphorylated at Ser-307 but not Ser-303. Transactivation assays matched the mapping results closely: substitution of Ser-307 but not of Ser-303 results in deregulation of the transcription function of HSF1. Apparently, peptide C needs to be phosphorylated in transcriptionally inactive HSF1. In various constitutively active mutants of HSF1 (LexA-HSF1), peptide C is not phosphorylated effectively, suggesting that dephosphorylation of the peptide is a hallmark of activated HSF1. These findings also imply that rephosphorylation of peptide C cannot trigger the return of the factor to an inactive state during recovery from heat stress, which kind of mechanism, i.e. desphosphorylation of HSF of the stress, has been suggested to play a role in the inactivation of yeast HSF (23). Extension of the analysis of the phosphorylation status of peptide C to additional deletion mutants suggested that most of or, perhaps, the entire region between residue 186 and the end of the HSF1 sequence plays a role in keeping HSF1 in a transcriptionally inert state, i.e. that much of the HSF1 sequence participates in the regulation of the transcription function, and that activation of HSF1 involves global changes in the structure of the molecule.
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MATERIALS AND METHODS |
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Cell Culture and [32P]Orthophosphate Labeling of Proteins-- Hela or Hela-CAT cells containing stably transformed chloramphenicol acetyltransferase (CAT) reporter genes controlled by the human hsp70B promoter (24) were grown in 100- or 60-mm dishes in Dulbecco's modified Eagle's medium (DMEM) with 10% fetal calf serum at 37 °C and 5% CO2. For experiments involving [32P]orthophosphate labeling of proteins, transfected (about 2 × 107 cells) or untransfected Hela-CAT cells (about 108 cells) were washed with phosphate-free DMEM, preincubated for 40 min in phosphate-free DMEM supplemented with 5% dialyzed calf serum, and then incubated for 2 h with [32P]orthophosphate (200 µCi/ml) at 37 °C prior to a 30-min heat treatment at 42-43 °C. Control cultures were labeled at 37 °C for 2.5 h.
Plasmids-- All LexA-HSF1 genes were under the control of the CMV promoter present in pcDNA vectors (Invitrogen). Construction of the LexA-HSF1 chimera and of all HSF1 deletions used herein was described previously (11, 22). HSF1 deletions were introduced into the chimera by standard subcloning procedures, making use of conveniently located restriction sites. Single or multiple amino acid substitutions were made by replacing short restriction fragments containing the sites to be mutated by corresponding fragments resulting from restriction digestion of polymerase chain reaction fragments into which the desired mutations had been introduced by means of appropriately designed primers. The presence of substitutions was verified by DNA sequence analysis.
Transfections--
Transfections were performed using the
LipofectAMINETM reagent (Life Technologies, Inc.). For
experiments involving [32P]orthophosphate labeling of
proteins, 70% confluent Hela-CAT cells in 100-mm dishes were incubated
for 5 h with 3 ml of a mixture containing 1 µg of a construct
containing a CMV promoter-driven -galactosidase reporter gene (22),
10 µg of a construct containing a LexA-HSF1 gene, and 15 µl of
LipofectAMINETM reagent in serum-free medium. Subsequent to
this incubation, cells were washed and incubated for about 40 h in
complete medium. For transactivation experiments, 70% confluent HeLa
cells in 60-mm dishes were used. Transfections were carried out as
before, except that cultures were incubated with a 1-ml mixture
including 1 µg of a LexA-HSF1 construct, 0.5 µg of a construct
containing a CAT reporter gene functionally linked to a minimal
promoter supplemented with LexA binding sites (LexA-CAT; Ref.11), and
0.5 µg of the CMV-
-galactosidase reporter gene construct.
Following transfection, cultures were incubated in complete medium for
15 h prior to heat treatment.
Enzyme Activity Assays--
CAT assays were performed as
described by Gorman et al. (25). -Galactosidase assays
employed a standard colorimetric procedure (6).
Immunoprecipitation of HSF1 or LexA-HSF1, and Phosphopeptide
Mapping--
Cells (about 2 × 107; about
108 cells in mapping experiments with endogenous HSF1),
[32P]orthophosphate-labeled as described before, were
collected and washed with phosphate-buffered saline. They were lysed in
0.4 ml of radioimmune precipitation buffer (50 mM Tris-HCl
(pH 7.5), 150 mM sodium chloride, 1% sodium deoxycholate,
1% Triton X-100, 5 mM sodium vanadate, 0.5 mM
sodium fluoride, 0.5 mM phenylmethylsulfonyl fluoride), and
the lysate was clarified by centrifugation. HSF1 or LexA-HSF1 was
immunoprecipitated in the cold from 400 µl of cleared lysate using a
previously described (1) rabbit anti-HSF1 polyclonal antibody bound to
protein A-Sepharose CL-4B. The immunoprecipitate was dissolved in
sample buffer and fractionated by 7.5% SDS-polyacrylamide gel
electrophoresis. The gel was dried and exposed to autoradiography. Regions containing HSF1 or LexA-HSF1 (or mutant derivatives) were excised, and the gel slices were dispersed in 1 ml of 50 mM
ammonium bicarbonate, pH 7.4. After addition of 50 µl of
-mercaptoethanol and 10 µl of 10% SDS, the mixture was boiled for
5 min and then incubated at room temperature for 3 h. Following
removal of gel pieces and addition of 20 µg of bovine serum albumin,
HSF1/LexA-HSF1 was precipitated with 20% trichloroacetic acid. The
pellet was washed with cold ethanol and taken up in ice-cold performic
acid, and the solution was incubated on ice for 1 h to oxidize
protein. After two cycles of lyophilization, oxidized protein was
dissolved in 50 µl of 50 mM ammonium bicarbonate, pH 7.4, and 2 µg of TPCK-trypsin were added. Proteinase digestion was for
15 h at 37 °C. TPCK-trypsin (2 µg) was added twice again over
the course of the reaction. After two cycles of lyophilization,
peptides were resuspended in electrophoresis buffer (1:3.5:40, formic
acid/glacial acetic acid/water (pH 1.9)) and, after addition of markers
(Tramine, Xylene cyanol FF, and
-DNP-lysine), were applied to
a cellulose TLC plate (EM Laboratories). Phosphopeptides were
separated in the first dimension by electrophoresis (1030 volts for 35 min at 15 °C) using an HTLE 7000 apparatus (C.B.S. Scientific) and in the second dimension by chromatography in n-butanol,
pyridine, glacial acetic acid, and water (5:3.3:1:4) (26). Radiolabeled phosphopeptides were detected by PhosphorImager (Molecular
Dynamics).
Phosphorylation of Peptides in Vitro--
For assays involving
protein kinase C, synthetic peptide (20 µg) corresponding to residues
295-311 of human HSF1 (VRVKEEPPSPPQSPRVE) was added to reaction
mixtures (50 µl) containing 20 mM MOPS, pH 7.2, 25 mM -glycerophosphate, 15 mM
MgCl2, 1 mM CaCl2, 1 mM sodium orthovanadate, 1 mM dithiothreitol, 90 µM ATP, 0.1 mg/ml diglycerides, 0.1 mg/ml
phosphatidylserine, 10 µCi [32P]ATP and 0.1 µg of
protein kinase C (mixture of
,
, and
isoforms from rat
brain). For MAP kinase assays, reaction mixtures (50 µl) contained 20 mM MOPS, pH 7.2, 25 mM
-glycerophosphate, 15 mM MgCl2, 5 mM EGTA, 1 mM sodium orthovanadate, 1 mM dithiothreitol, 90 µM ATP, 20 µg of peptide, 10 µCi
[32P]ATP, and 0.2 µg of recombinant, active p44 Erk1 or
0.1 µg of recombinant, active p42 Erk2. All protein kinases were from
Upstate Biotechnology. Following incubation at 30 °C for 1 h,
peptides were precipitated with 20% trichloroacetic acid in the
presence of 20 µg of bovine serum albumin. Precipitates were washed,
dissolved, digested with trypsin, and thin layer-electrophoresed and
chromatographed as described in the previous section.
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RESULTS |
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LexA-Human HSF1 Expressed from Transfected Genes Is Similarly Hyperphosphorylated as Endogenous Human HSF1-- To radiolabel phosphorylatable residues in HSF1, HeLa-CAT cells were incubated for 2 h at 37 °C and then for an additional 30 min either at 42-43 °C (heat shock) or at 37 °C (control) in the presence of [32P]orthophosphate. Cells were collected and lysed in the presence of phosphatase and protease inhibitors, and HSF1 was immunoprecipitated with an HSF1-specific antibody, subjected to SDS-polyacrylamide gel electrophoresis, eluted from the gel, carefully oxidized, and digested to completion with trypsin. Peptides were resolved by thin layer electrophoresis and chromatography, and radiolabeled peptides were detected by a PhosphorImager, resulting in the two-dimensional maps shown in Fig. 1, A and B. Similar patterns of HSF1 phosphopeptides (labeled A through D) were obtained with heat-shocked and control cells. Heat shock increased apparent phosphorylation (see "Discussion") of all HSF1 peptides severalfold.
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HSF1 Appears to be Phosphorylated on Ser-307 but Not Effectively on Ser-303-- When HeLa-CAT cells (transfected with a functional HSF1 gene to enhance effects) are exposed to 42 °C for 30 min, they respond by synthesizing a modest quantity of CAT. Preexposure of the cells to phorbol ester greatly enhances (5.4-fold) this response (17). The simplest interpretation of this finding is that phosphorylation by a protein kinase C stimulates the transcriptional activity of HSF1. This notion is also supported by the observation that various inhibitors of protein kinase C inhibit heat-induced hyperphosphorylation of HSF1 (17). Protein kinase A was previously suggested to play a role in HSF regulation (27). A search for consensus protein kinase sites in the HSF1 sequence suggested that Thr-120, Thr-124, Ser-174, Ser-199, and Ser-307 could be targets for phosphorylation by protein kinase C, and Thr-120 also for protein kinase A. (The numbering is identical to that used by Rabindran et al. (28)).
A set of LexA-HSF1 chimeras was prepared in which one or two of these residues were substituted with alanine. The mutations were combined to create chimeras carrying multiple mutations. A chimera containing all five mutations was subjected to phosphopeptide mapping as described before (Fig. 2A). The resulting phosphopeptide pattern was similar to that of the original unmutated chimera except for the absence of phosphopeptide C. When the transcriptional abilities of chimeras with different mutations were tested in HeLa cells (using the transactivation assay described below), it was observed that, unlike the unmutated chimera, chimeras including an alanine substitution of Ser-307 (S307A) were active at non-heat shock temperature (not shown). Based on these results, it was tentatively concluded that the absence of a phosphorylated residue at position 307 resulted in deregulation of the chimeric HSF1, and that phosphopeptide C corresponded to peptide VKEEPPSPPQSPR (297-309) phosphorylated at Ser-307. Confirmation was obtained from a mapping experiment with a LexA-HSF1 chimera with a single alanine substitution at Ser-307 (S307A; Fig. 2B). As expected, phosphopeptide C was virtually absent from the map. Surprisingly, phosphopeptide A was also absent, and new phosphopeptide A' appeared. Since phosphopeptides A and A' have similar chromatographic properties, and A' migrates twice as far as A in the electrophoretic dimension, it is probable that phosphopeptides A and A' are identical except that phosphopeptide A is phosphorylated on two residues and A' on only one. Phosphorylation of one of the two phosphorylatable residues in peptide A may be dependent on a conformational change brought about by phosphorylation of Ser-307. The above result also indicates that phosphorylation of Thr-120, Thr-124, Ser-174, and Ser-199 does not contribute to the phosphopeptides appearing in the map of LexA-HSF1.
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Phosphorylation of Peptide C Is Drastically Reduced in Activated HSF1-- To find out whether activation of HSF1 is accompanied by a change in phosphorylation of peptides A-D, several deletions and substitutions known to be active in the absence of stress were subjected to phosphopeptide mapping. Exemplary results from transactivation assays and phosphopeptide mapping experiments with three mutants are shown in Table I and Fig. 4, respectively. The map of the large deletion LexA-HSF1d202-316 was found to lack phosphopeptides A, C, and D (Fig. 4A). The absence of phosphopeptide C is expected since Ser-307 lies within the region deleted from this mutant factor. A much reduced phosphopeptide C signal was also noted in the map of the small deletion LexA-HSF1d186-202 (Fig. 4B). The map of S275A reveals phosphorylation of peptides A and B, but peptide C is virtually unphosphorylated (Fig. 4C). A quantitative analysis of these observations is presented in Table I. Analogous results were obtained with two additional constitutively active mutants (d202-277 and S279A/S283A; not shown). Thus, the common feature of the maps of all five mutants analyzed is a much reduced intensity of the phosphopeptide C signal, suggesting that peptide C cannot be phosphorylated effectively in the activated HSF1 molecule. No consistent differences in the phosphorylation of the other peptides were observed: the absence of phosphopeptide A does not correlate with deregulation of factor activity (compare maps of LexA-HSF1, d202-316, S307A, and S303A/S307A), and phosphopeptide B is present in all maps. No definitive answer was obtained regarding changes in phosphorylation of peptide D because of the low intensity of the phosphopeptide D signal that made it difficult to ascertain its absence from some of the maps.
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Carboxyl-terminal Sequences Appear to Play a Role in Maintaining HSF1 in an Inactive Conformation-- It follows from the experiments discussed before that the phosphorylation status of peptide C can serve as an indicator of the conformational (i.e. inactive versus active) state of HSF1. Assays of phosphorylation of this peptide were used to find out whether sequences far removed from the regulatory domain could affect the conformational state of HSF1. To this end, phosphopeptide maps were obtained for deletions LexA-HSF1d453-523 and d409-465. The two mutants produced maps (Figs. 4, D and E, see also Table I) that were similar to that of LexA-HSF1, except for a much reduced intensity of phosphopeptide C signal. Thus, it appears that deletion of sequences located near the carboxyl-terminal end prompts HSF1 to assume an activated conformation. These results suggest that sequences far removed from the regulatory domain participate in the maintenance of the inactive state of the factor.
On the Location of Other Phosphorylatable Sites-- The location of the phosphorylated residues in peptides A, B, and D has not yet been determined definitively. Analysis of deletions LexA-HSF1d453-523 (Fig. 4A) and d409-465 (Fig. 4, D and E) places all three peptides amino terminal from residue 381. Based on the map of LexA-HSF1dd202-316 (Fig. 4A), peptides A and D may originate from the region deleted from this mutant, i.e. from the regulatory region of HSF1.
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DISCUSSION |
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Similar patterns of 32P-labeled tryptic phosphopeptides were obtained with HSF1 from non-stressed HeLa cells and from cells that had been exposed to a moderate heat stress. Heat treatment greatly enhanced radiolabeling of the peptides. Several different mechanisms could account for this effect. First, the peptides may be incompletely phosphorylated under non-stress conditions, and heat stress may cause them to become fully phosphorylated (first mechanism). In a second mechanism, target residues may be continuously phosphorylated and dephosphorylated, and the turnover rate may increase with temperature. A third mechanism may be provided by the transient nature of HSF1 activation. Under conditions of moderate heat shock, both activation and inactivation reactions occur at signficant rates; while the activation reaction predominates initially, the balance changes in favor of the inactivation reaction with time, a phenomenon known as attenuation (29). Residues in HSF1 that are phosphorylated under non-shock conditions but dephosphorylated during heat activation would be rephosphorylated to some extent in the course of a moderate heat stress, resulting in incorporation of 32P04. Different mechanisms may be responsible for incorporation of radioactivity into different tryptic peptides. Our studies suggest that 32P labeling of peptide C occurs by the third mechanism. At least one of the four peptides identified is expected to be 32P-labeled according to the first mechanism; in Western blots of extract from non-stressed cells, HSF1 appears as several bands in the 70-80 kDa molecular mass range. When extract from heat-shocked cells is analyzed, a similar pattern of bands is observed, but the abundance of the most slowly migrating bands is increased drastically relative to the faster migrating forms, indicating a heat-induced shift to more highly phosphorylated HSF1 species. The fact that this shift in distribution can be observed by Western blot implies that heat-induced phosphorylation events occur in most HSF1 molecules. Since inducible phosphorylation involves addition of a radiolabeled phosphate group to a previously unphosphorlyated residue during heat shock, the specific radioactivity of a phosphopeptide including a newly phosphorylated residue should be at least equal to or higher than that of a phosphopeptide containing a residue 32P-labeled by turnover or during recovery. Thus, a truly inducibly phosphorylated peptides should be represented by one of the major signals present in our maps.
Two previous studies highlighted the importance of phosphorylation at Ser-303 (16, 21), and a third did not discriminate between phosphorylation of Ser-303 and Ser-307 (20). The study by Chu et al. (21) relied mostly on in vitro phosphorylation experiments. It showed that incubation of recombinant HSF1 with MAP kinase results in molecules phosphorylated on Ser-307 and that the latter molecules can be further phosphorylated on Ser-303 by glycogen synthase kinase 3. The significance of these observations remains unknown. The study by Kline and Morimoto (16) detected in excess of ten tryptic phosphopeptides originating from HSF1 32P-labeled in vivo. The specific radioactivity of about half of these phosphopeptides was increased modestly (the "constitutive phosphopeptides") and of the other half increased more drastically (the "inducible phosphopeptides") during heat treatment. A similar phosphopeptide pattern was observed for a GAL4-mouse HSF1d1-123 chimera expressed in COS monkey cells. The same experimental system was then used to produce maps of similar chimeras containing additional deletions or substitutions in the HSF1 sequence. Substitution in the original chimera of Ser-303 and Ser-307 led to the disappearance of four of the five major constitutive phosphopeptides. Substitution of either Ser-303 or Ser-307 deleted three of the same four phosphopeptides. In functional assays, S303A and S303A/S307A substitutions were found to be constitutively active. A single substitution of Ser-307 was not tested. Ser-303 and Ser-307 lie within the same tryptic peptide (referred to herein as peptide C). Thus, even if phosphorylation of these residues was incomplete, thin layer electrophoresis and chromatography could only distinguish singly and doubly phosphorylated peptide C, i.e. no more than two signals should be attributable to the peptide. As we pointed out, the appearance of four different signals originating from peptide C is indicative of some technical problem with the preparation of phosphopeptides. Presumably because oxidation and proteolytic cleavage reactions ran to completion in our experiments, the resulting maps revealed a much simpler pattern, consisting of only four major signals. S303A/S307A and S307A substitutions led to the disappearance of phosphopeptide C. These findings support the conclusion that peptide C is identical with peptide VKEEPPSPPQSPR (297-309), containing Ser-303 and Ser-307. In contrast, phosphopeptide C still was present as a major signal in the map of an S303A substitution, suggesting that phosphopeptide C is singly phosphorylated on Ser-307. In transactivation assays, S307A and S303A/S307A substitutions were deregulated, whereas an S303A substitution was normally heat-regulated. We conclude from these results that Ser-307 but not Ser-303 is phosphorylated and suggest that phosphorylation of Ser-307 plays a regulatory role. Although the observation (discussed more fully below) that active HSF1 is underphosphorylated further supports a regulatory role of Ser-307 phosphorylation, it is noted that the alternative interpretation of our transactivation assays with the S307A substitution mutant, which is that the substitution itself resulted in an activating conformational change, cannot be categorically ruled out.
As discussed before (in the Introduction), the substrate for stress-inducible phosphorylation most likely is the HSF1 trimer. Constitutive phosphorylation may occur in either or both, non-trimeric and trimeric, inactive HSF1. While the question which of these forms of HSF1 is the true substrate for constitutive phosphorylation may not be easily resolved, it may not be critical from a practical point of view. Similar phosphopeptide patterns were obtained with (endogenous) HSF1 from unstressed (HSF1 largely monomeric) and stressed (HSF1 largely trimeric prior to phosphorylation) cells. The present study employed LexA-HSF1 chimeras that are trimeric under the experimental conditions used and are regulated identically with wild-type HSF1 (11, 22). In contrast, the Kline and Morimoto study (16) was performed with GAL4-HSF1 molecules that include the dominant dimerization domain of GAL4 in addition to or instead of the HSF1 trimerization domain. Presumably, the GAL4-HSF1 chimeras are dimeric, and the HSF1 sequences contained in the chimeras fold improperly because of the presence of HSF1 trimerization domains that are unable to assemble into a trimeric structure or because of the lack of these domains, as the case may be. In the resulting, atypically folded chimera, but not in native HSF1, Ser-303 may become a target of phosphorylation, and phosphorylation of this residue that lies in the regulatory region of the molecule may affect the functional properties of the chimera.
Phosphorylation of HSF1 is influenced by conformational changes in the molecule. Whereas endogenous HSF1 and the wild-type and S303A chimeras produce an intense phosphopeptide C signal, this signal is either weak or absent in constitutively active mutants (d186-202, d202-277, d202-316, S275A and S279A/S283A). This observation suggests that peptide C, i.e. Ser-307, is only phosphorylated when HSF1 is in an inactive conformation but not when it is in the active conformation. Presumably, phosphoserine 307 is dephosphorylated in the course of HSF1 activation. Since phosphorylation of Ser-307 apparently cannot occur in the active conformation, this event is unlikely to play a pivotal role in the inactivation of the factor subsequent to a stressful event. Rather, Ser-307 may be rephosphorylated after active HSF1 has been converted to an inactive form by another mechanism. In contrast, as substitution of Ser-307 by a non-phosphorylatable amino acid suffices to activate HSF1, it is conceivable that dephosphorylation of phosphoserine 307 is an intermediate step in the activation of the factor. Alternatively, dephosphorylation of the residue may serve to stabilize the activated conformation of HSF1. Note that because phosphoserine 307 is likely to be dephosphorylated during heat shock, heat-inducible incorporation of [32P]orthophosphate at Ser-307 may be best explained by the third mechanism discussed before (involving rephosphorylation of the residue in the presence of 32P04 subsequent to dephosphorylation).
Finally, advantage was taken of the observation of a close correlation between activation of HSF1 and dephosphorylation of phosphoserine 307 to ask whether mutations in HSF1 sequences distal to the regulatory domain (located between residues 186 and 315) also cause the factor to acquire an active conformation. The region near the carboxyl terminus of the 529-residue-long HSF1 sequence contains at least two activation domains (15). Somehow the conformational state of the regulatory domain determines whether or not the distant activation domains are functional. One possible mechanism by which this regulation at a considerable distance (100-300 residues) could be achieved would involve an interaction (direct or via an intermediary protein) between the regulatory domain and the activation domains, an interaction which is disrupted in the course of activation. A related mechanism may involve interactions between the activation domains and sequences preceding the regulatory domain. If one of these mechanisms were regulating the activation domains, one would predict that certain mutations in either the regulatory domain or the activation domains could cause the factor to assume an activated conformation. While this is clearly the case for the regulatory domain as shown by the ability of HSF1 molecules mutated in the regulatory domain to transactivate a reporter gene in the absence of stress, it has not been possible to similarly analyze the activation domains for obvious reasons. Our results suggested that dephosphorylation of phosphoserine 307 can serve as an indicator of the active conformation that is independent of the factor's transcriptional activity, providing us with a tool for examining the regulatory influence of carboxyl terminal located HSF1 sequences. We found that a deletion mutant lacking the carboxyl-terminal end of HSF1 (d453-523) and an internal deletion (d409-465) produced maps with drastically reduced Ser-307 (phosphopeptide C) signals. These observations support a model of regulation in which the regulatory region and carboxyl-terminal located sequences including the activation domains are involved in establishing an inactive conformational fold that includes over half of the sequence of HSF1. The phosphopeptide mapping approach may be used to further delineate elements located in the carboxyl half of the HSF1 sequence that participate in the regulatory mechanism.
Note that the assignment of Ser-307 as a phosphorylation target, although fully supported by the available evidence, cannot be made with absolute certainty. One of the observations made in the present study is that activated HSF1 mutants or carboxyl-terminal deletions produce a much reduced phosphopeptide C signal. This finding raises the possibility that a single amino acid substitution may alter HSF1 conformation to such an extent that dephosphorylation of phosphopeptide C is sufficiently accelerated to reduce the level of 32P-labeled phosphopeptide C to below the limit of detection.
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ACKNOWLEDGEMENTS |
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We thank Jiangying Zou and Rong Xu for assistance with the art work.
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FOOTNOTES |
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* These studies were supported by Grant GM31125 from the NIGMS, National Institutes of Health (to R. V.).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.
Present address: Division of Hematology-Oncology, Dept. of
Medicine, University of Miami School of Medicine, 1475 NW 12th Ave.
(D8-4), Miami, FL 33136.
§ Present address: Laboratory of Plant Molecular Biology, The Rockefeller University, 1230 York Ave., New York, NY 10021.
¶ To whom correpondence should be addressed: Dept. of Biochemistry and Molecular Biology, University of Miami School of Medicine, P. O. Box 016129, Miami, FL 33101-6129 (1011 NW 15th St., Miami, FL 33136-1015). Tel.: 305-243-5816; Fax: 305-243-3064.
1 The abbreviations used are: hsp, heat shock protein; HSF, heat shock factor; HSE, heat shock element; MAP, mitogen-activated protein; CAT, chloramphenicol acetyltransferase; DMEM, Dulbecco's modified Eagle's medium; CMV, cytomegalovirus; TPCK, L-1-tosylamido-2-phenylethyl chloromethyl ketone; TLC, thin layer chromatography; MOPS, 4-morpholinepropanesulfonic acid; MEK-1, extracellular signal-regulated kinase kinase-1.
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