Acetylation at Lysine 183 of Progesterone Receptor by p300 Accelerates DNA Binding Kinetics and Transactivation of Direct Target Genes

Background: The identification of steroid receptor acetylation was based on the consensus motif (K/R)XKK. Results: Mass spectrometry discovers PR acetylation at non-consensus lysine 183 by p300. Lys-183 acetylation enhances PR-DNA binding kinetic and transcription activity. Conclusion: PR acetylation at Lys-183 promotes PR-gene enhancer interaction. Significance: The study provides a novel insight into the regulation of PR function by acetylation. The identification of lysine acetylation of steroid hormone receptors has previously been based on the presence of consensus motif (K/R)XKK. This study reports the discovery by mass spectrometry of a novel progesterone receptor acetylation site at Lys-183 that is not in the consensus motif. In vivo acetylation and mutagenesis experiments revealed that Lys-183 is a primary site of progesterone receptor (PR) acetylation. Lys-183 acetylation is enhanced by p300 overexpression and abrogated by p300 gene silencing, suggesting that p300 is the major acetyltransferase for Lys-183 acetylation. Furthermore, p300-mediated Lys-183 acetylation is associated with heightened PR activity. Accordingly, the acetylation-mimicking mutant PRB-K183Q exhibited accelerated DNA binding kinetics and greater activity compared with the wild-type PRB on genes containing progesterone response element. In contrast, Lys-183 acetylation had no influence on PR tethering effect on the nuclear factor κ-light chain enhancer of activated B cells (NFκB). Additionally, increases of Lys-183 acetylation by p300 overexpression or inhibition of deacetylation resulted in increases of Ser-294 phosphorylation levels. In conclusion, PR acetylation at Lys-183 by p300 potentiates PR activity through accelerated binding of its direct target genes without affecting PR tethering on other transcription factors. The effect may be mediated by enhancing Ser-294 phosphorylation.

The ovarian steroid hormone progesterone is essential for normal mammary and uterine development. It is also imperative for embryo implantation and maintenance of pregnancy. The progesterone receptor (PR) 2 is the principal mediator of progesterone action. There are two major subtypes of human PR, PR-A and PR-B, that are translated from transcripts generated from two distinct promoters in the gene (1). PRA lacks the 165 amino acids found in the N terminus of PRB. PR isoforms are differentially expressed in a cell-or tissue-specific manner (2)(3)(4). PR belongs to the nuclear receptor superfamily that is characterized by a modular domain structure. The structure of PR begins with a poorly conserved N-terminal transactivation domain (NTD) that includes the activation function-1 (AF-1) originally defined to a core region of amino acids 456 -546 (5). This is followed by the DNA binding domain responsible for receptor dimerization and DNA binding. The C-terminal ligand binding domain contains AF-2. AF-1 synergizes with AF-2 to bring about optimal receptor activity (6). In addition, an AF-3 is contained within the first 164 amino acids unique to PRB and synergizes with both AF-1 and AF-2 to maximize PRB activity. There is also a flexible hinge region, connecting the DNA binding domain and ligand binding domain (7). Hinge region contains the nuclear localization signal. It has been reported that PR hinge region also plays a role in regulating PR transactivation through its acetylation (8).
The PR function is regulated by a host of transcription coregulators. Agonist binding results in a conformational change in the ligand binding domain that allows the receptor to interact directly or indirectly with a diverse set of co-regulatory proteins (7). These include steroid receptor coactivator (SRC) family members (i.e. SRC-1, SRC-2, and SRC-3), which act primarily as anchoring surfaces to bridge the binding of other coregulators, such as protein-modifying enzymes acetyltransferases and methyltransferases (9 -13). p300, its paralog CREBbinding protein (CBP), and p300/CBP-associated factor (PCAF) are the best characterized mammalian acetyltransferases. These proteins co-regulate the activities of a variety of transcription factors, including PRs and other nuclear receptors (14 -21). They are recruited to PR in a ligand-dependent manner via interactions with SRC proteins (13) and acetylate nucleosomal histones and transcription coregulators to modulate transcriptional activity (22). For example, acetylation could facilitate recruitment of transcription factors to specific target DNA sequences by loosening nucleosomal structure and facilitate transcription factor binding to gene promoters. In addi-tion, p300 and CBP can also directly acetylate nuclear receptors to regulate their transcriptional activity (20,23,24). Although it has been reported that p300 is associated with PR during progesterone-induced transcriptional initiation (13), it is not known whether p300 directly acetylates PR to regulate its activity. Nonetheless, it has been reported that PR is acetylated at the consensus sequence, KXKK (amino acids 638 -641) of the hinge region (8). This PR acetylation was hormone-inducible and was able to regulate the kinetics of transcription of fast response genes and transcription magnitude of slow response genes (8).
Using LC-MS/MS analysis of immunoprecipitated PR from breast cancer cell lines T47D and ABC28, we have uncovered a novel acetylated site (Lys-183) of high confidence located in the N-terminal domain of PR. Using various biochemical and cellbased assays, we have validated that Lys-183 is the major target of PR acetylation by p300. In addition, we explored the mechanisms and functional consequences of Lys-183 acetylation and demonstrated that Lys-183 acetylation specifically enhances PR transactivation of genes containing PRE. Such regulation is likely to be important in modulating progesterone-dependent signaling in a variety of progesterone target tissues in both normal and pathological states.

EXPERIMENTAL PROCEDURES
Cell Culture-MDA-MB-231, COS7, and HeLa cell lines were obtained from American Type Culture Collection (ATCC, Manassas, VA). ABC28 clone was derived by transfecting MDA-MB-231 cells with PR expression vectors hPR1 and hPR2 that contain human PR cDNA coding for PR isoform B and isoform A in pSG5 plasmid (25). Cells were routinely maintained in phenol red Dulbecco's modified Eagle's medium (DMEM) supplemented with 7.5% fetal calf serum (FCS) (Sigma-Aldrich) and 2 mM L-glutamine at 37°C in a humidified atmosphere of 5% CO 2 , 95% air. For experiments involving hormone treatment, cells were cultured in phenol red-free DMEM supplemented with 5% charcoal-stripped FBS and 2 mM L-glutamine for 2 days prior to treatment with progesterone, RU486, or R5020 (Sigma-Aldrich).
Protein Lysate Collection and Western Blotting Analysis-Cells were lysed with cold lysis buffer (50 mM HEPES, 150 mM NaCl, 1% Triton X-100, 5 g/ml pepstatin A, 5 g/ml leupeptin, 2 g/ml aprotinin, 1 mM PMSF, 100 mM sodium fluoride, and 1 mM sodium vanadate (pH 7.5)), and proteins in the supernatant were collected after centrifugation at 12,000 ϫ g for 12 min at 4°C. Protein concentration was determined using the BCA TM protein assay kit (Pierce). Proteins were resolved by SDS-PAGE before transferring onto a nitrocellulose membrane (Amersham Biosciences). Anti-PR antibody, H-190 (Santa Cruz Biotechnology, Inc.) was used to probe for human PR isoforms, PR-A and PR-B. Phospho-Ser-294 was probed by Ser-294 antibody from Neomarkers. Acetylated proteins were detected by a pan-anti-acetylated lysine antibody (Cell Signaling). The secondary anti-mouse and anti-rabbit antibodies (GE Healthcare) were used in dilutions of 1:1000 and 1:2000, respectively, in reference to the primary antibody used. Anti-␤-actin (Santa Cruz Biotechnology) was used to probe for ␤-actin as loading control. Signal detection was carried out using enhanced chemiluminescence (ECL) (GE Healthcare) or Immobilon Western Chemiluminescent HRP substrate (Millipore) according to the manufacturer's protocol on x-ray films (Eastman Kodak Co.).
PR Immunoprecipitation-For MS identification of PR acetylation, ABC28 cell lysates were prepared in lysis buffer and incubated overnight at 4°C with anti-PR antibody (H-190, Santa Cruz Biotechnology) precaptured by protein A/G-agarose beads (Santa Cruz Biotechnology). The immune complexes were subsequently washed two times with lysis buffer and two more times with high salt (500 mM NaCl) lysis buffer to remove nonspecific binding. Bound proteins were eluted by boiling in Laemmli sample buffer. The immunoprecipitated proteins were resolved by SDS-PAGE, fixed, and stained by Coomassie Blue G-250 (Sigma-Aldrich).
In-gel Tryptic Digestion-The PR gel bands were excised, chopped into small pieces (ϳ1 ϫ 1 mm), and transferred to Eppendorf tubes. They were washed with Milli-Q water; destained with 50% acetonitrile (ACN), 50% 25 mM NH 4 HCO 3 via vigorous vortexing for 30 min three times; and dehydrated with 100% ACN until the gel particles became white. They were then reduced with 10 mM dithiothreitol (DTT) at 56°C for 1 h and alkylated with 55 mM indoacetamide for 45 min in the dark followed by successive washes with 25 mM NH 4 HCO 3 and 50% ACN, 50% 25 mM NH 4 HCO 3 . Finally, they were dehydrated with 100% ACN and dried in vacuum. Trypsin (Trypsin Gold, Mass Spectrometry Grade, Promega, Madison, WI) was added in a weight ratio of 1:30. After the trypsin solution was completely absorbed by gel particles, 25 mM NH 4 HCO 3 was added to completely cover the particles. They were then incubated at 37°C overnight. Tryptic peptides were extracted from gel particles with 50% ACN containing 0.1% formic acid under sonication for 2 ϫ 20 min. The combined extracts were dried in vacuum.
LC-MS/MS and Data Analysis-LC-MS/MS was carried out as described previously (26). Briefly, peptides were separated and analyzed on a liquid chromatograph (Dionex UltiMate 3000 Nano-LC Systems) at a 300-nl/min flow rate coupled to an LTQ-FT Ultra system (Thermo Electron, Bremen, Germany). Mobile phase A (0.1% formic acid in H 2 O) and mobile phase B (0.1% formic acid in ACN) were used to establish the 60-min gradient composed of 45 min of 5-35% B, 8 min of 35-50% B, and 2 min of 80% B followed by re-equilibration at 5% B for 5 min. Peptides were then analyzed on the LTQ-FT system with an ADVANCE TM CaptiveSpray TM source (Michrom BioResources) at an electrospray potential of 1.5 kV. A gas flow of 2, ion transfer tube temperature of 180°C, and collision gas pressure of 0.85 millitorrs were used. A full MS scan (350 -1600 m/z range) was acquired in the FT-ICR cell at a resolution of 100,000 and a maximum ion accumulation time of 1000 ms. The automatic gain control target for FT was set at 1eϩ06, and precursor ion charge state screening was activated. The linear ion trap was used to collect peptides and to measure peptide fragments generated by collision-induced dissociation. The default automatic gain control setting was used (full MS target at 3.0eϩ04, MS n at 1eϩ04) in the linear ion trap. The 10 most intense ions above a 500-count threshold were selected for fragmentation in collision-induced dissociation (MS 2 ), which was performed concurrently with a maximum ion accumulation time of 200 ms. For collision-induced dissociation, the activation Q was set at 0.25, isolation width (m/z) was 2.0, activation time was 30 ms, and normalized collision energy was 35% (27).
The MS/MS spectra in the raw data were first extracted into the dta format using the extract_msn (version 4.0) in Bioworks Browser (version 3.3, Thermo Fisher Scientific), and then the dta files were converted into the Mascot generic file format using an in-house program. Intensity values and fragment ion m/z ratios were not manipulated. The Uniprot human protein database (downloaded on April 5, 2013, with 132,655 sequences; 43,940,360 residues) was used for database searches. The database search was performed using an in-house Mascot server (version 2.4.0, Matrix Science, London, UK) with MS tolerance of 10 ppm, option 13 C of 2, and MS/MS tolerance of 0.8 Da. Two missed cleavage sites of trypsin were allowed. Carbamidomethylation (Cys) was set as a fixed modification, and oxidation (Met), deamidation (Asn-Gln), acetylation (Lys), methylation (Lys-Arg), dimethylation (Lys-Arg), and trimethylation (Lys) were set as variable modifications. The obtained database search results were exported to Microsoft Excel using the export_dat_2.pl script of Mascot for further analysis. Only peptides with E-values of less than 0.05 and Mowse scores greater than the identity or homology scores were further manually analyzed.
PR Mutant Construction by Site-directed Mutagenesis-pcDNA3.1 expression vectors encoding human PRB have been described previously (28). Point mutations of the Lys residue at site 183 of PR to glutamine and arginine were generated using the QuikChange XL site-directed mutagenesis kit (Stratagene) according to the manufacturer's protocol. The site-directed primers were designed using a Web-based program known as QuikChange Primer Design. The mutations were verified by fulllength cDNA sequencing. The sequences of mutagenic sense and antisense primers used were as follows: K183Q_sense, 5Ј-cgg cag ctg ccc atc agg tgc tgc ccc gg-3Ј; K183Q_antisense, 5Ј-ccg ggg cag cac ctg atg ggc agc tgc cg-3Ј; K183R_sense, 5Ј-gga cgg cag ctg ccc ata gag tgc tgc cc-3Ј; K183R_antisense, 5Ј-ggg cag cac tct atg ggc agc tgc cgt cc-3Ј.
Plasmid Transfection-COS7 or HeLa cells were plated in 35-mm dishes at a density of 2.5 ϫ 10 5 cells in antibiotic-free phenol red-free DMEM. The cells were then transfected with 0.5 g of pc-DNA3.1, pc-DNA3.1wt-PRB, or the various pc-DNA3.1 Lys-183-PRB mutants using polyethyleneimine (PEI) (CELLnTEC, Switzerland) after 24 h of plating. The cells were then treated with 0.1% ethanol, 10 nM R5020 for 1 h at 24 h post-transfection. The cell lysate was then collected to test for the expression of total PR and phospho-PR.
In Vitro Histone Acetyltransferase Assays of PR Peptides and PR Protein-The in vitro acetylation assay was carried out as described (24) with minor modifications. PR peptide (KVGDS-SGTAAAHK 183 VLPRGLSPARQL (wild type) or KVGDSSGT-AAAHQ 183 VLPRGLSPARQL (K3 Q))), 1 g of recombinant histone H3 protein (as positive control), or immunoprecipitated PR was incubated with 0.25 Ci of [ 3 H]acetyl coenzyme A (CoA) (Amersham Biosciences) and 100 ng of recombinant p300 enzyme (Active Motif) in 30 l of acetylation buffer containing 50 mM Tris (pH 8.0), 5% glycerol, 0.1 mM EDTA, 50 mM KCl, 1 mM DTT, 1 mM PMSF, and 10 mM sodium butyrate. Immunoprecipitated HA-CBP or FLAG-PCAF were also tested for their activity in acetylating PR in in vitro acetylation experiments. Reaction mixtures were incubated at 30°C for 1 h, stopped by the addition of 5ϫ Laemmli buffer, and resolved by SDS-PAGE. The reactions were analyzed first by Coomassie Blue staining to verify the amounts of proteins used in each reaction, and the same gel was subsequently subjected to autoradiography to evaluate acetylation.
In Vivo Acetylation Assay-The in vivo acetylation assay was carried out as reported (8). Briefly, PR-deficient COS7 cells were grown in DMEM containing 7.5% FBS and were transfected with pcDNA3.1-FLAG-PR in the presence or absence of pCI-FLAG-p300 using PEI. The transfected COS7 cells were pretreated with 10 M TSA for 30 min followed by vehicle control or 10 nM R5020 treatment for another 1 h before cell lysate collection. Protein lysate was collected for PR immunoprecipitation by FLAG antibody, and captured FLAG-PR and FLAG-p300 were resolved by SDS-PAGE. Acetylated proteins were probed by a pan-anti-acetylated lysine antibody (catalog no. 9441, Cell Signaling).
PR Luciferase Reporter Assay-Luciferase assay procedures were adapted from the manufacturer's protocol provided for the Dual-Luciferase Reporter System kit (Promega). Briefly, HeLa cells were seeded onto 60-mm dishes and were transfected with PEI with 5 ng of pcDNA3.1, pcDNA3.1-WT-PRB, or pcDNA3.1-PRB-K183Q/R in addition to 1500 ng of reporter plasmids, such as PRE-Luc reporter or NFB-Luc reporter. 1 ng of Renilla pRL-CMV vector was co-transfected as normalization control. 24 h post-transfection, the cells were treated with 0.1% EtOH or 10 nM R5020 for 12 h before the were lysed by 1ϫ passive lysis buffer provided in the Dual-Luciferase Reporter System kit (Promega). 20 l of lysate were analyzed using a computer-controlled microplate luminometer (Thermo Scientific Fluoroskan Ascent FL). The activities of the Renilla and firefly luciferase were measured according to the manufacturer's protocol. PRE/NFB-dependent luciferase activity was normalized by Renilla reading and expressed as the average relative light units (RLU) of triplicate or four replicate measures Ϯ S.E. -Fold induction by ligand was calculated as the ratio of ligand-induced sample RLU to the corresponding vehicle control-treated sample RLU.

Relative expression
After the amplification process, a melting curve analysis using the LightCycler instrument was performed to verify the specificity of the PCR products.
Chromatin Immunoprecipitation-Chromatin immunoprecipitation (ChIP) analyses were performed with procedures modified from protocols described previously (29). The ABC28 cell line was grown in DMEM supplemented with 5% dextran charcoal-stripped FBS for 3 days. Cells were then treated with R5020 (10 Ϫ8 M) for various durations, as indicated in the figure legends, before collection for the ChIP assay. Cells were fixed with formaldehyde at a final concentration of 1% for 10 min at room temperature; cross-linking was stopped by the addition of glycine to a final concentration of 0.125 M. Cells were then harvested, and the remaining steps followed standard protocols for ChIP experiments. Anti-PR antibody (H-190, Santa Cruz Biotechnology) was used for ChIP assays. PCR was performed to analyze immunoprecipitated chromatin in studies with ABC28 cells. The steps of PCR were as follows: 34 cycles with 1 min of denaturing at 94°C, annealing at 60°C, and extension at 68°C. After DNA purification (Geneaid), immunoprecipitated DNA was assayed for the binding of the human FKBP5 (FK506-binding protein 5) gene promoter sequences. Primers for the human intronic PRE region were as follows: sense, 5Ј-taa tag agg ggc gag aag gca ga-3Ј; antisense, 5Ј-ggt aag tgg gtg tgc tcg ctc a-3Ј. PCR products were analyzed by agarose gel (2%) electrophoresis.
Plasmid Immunoprecipitation-Plasmid immunoprecipitation experiments were performed as described previously with minor modifications (30). HeLa cells were grown in DMEM supplemented with 5% charcoal-dextran-stripped serum for 1 day and transfected with 10 ng of WT PRB or PRB-K183Q/R expression vectors, in addition to 1.5 g of PRE2-TATA luciferase reporter plasmid and/or 100 ng of PCI-FLAG-p300 or PCI vector control. 24 h post-transfection, cells were treated with either R5020 (10 Ϫ8 M) or vehicle control (0.01% EtOH) for various durations. Cross-linking and termination of cross-linking of cells were as described for the ChIP assay. Cells were then harvested, and the remaining steps followed standard protocols for ChIP experiments. Anti-PR antibody (H-190, Santa Cruz Biotechnology) was used for PR-PRE2-TATA-luciferase plasmid immunoprecipitation. The resulting immunoprecipitated and input DNA was analyzed by PCR or real-time PCRs with the following pair of primers for the detection of PRE luciferase sequences: sense, 5Ј-cta gca aaa tag gct gtc cc-3Ј; antisense, 5Ј-tat gtt ttt ggc gtc ttc cat-3Ј. PCR products were analyzed by 2% agarose gel electrophoresis.
Statistical Analysis-Data were analyzed using unpaired, two-tailed Student's t test with a 95% confidence interval using the program GraphPad Prism version 5.

Identification of PR Acetylation at Lys-183 by LC-MS/MS-
To further elucidate the mechanisms of progesterone action, sensitive LC-MS/MS tools were exploited to identify novel PR post-translational modifications using PR-transfected MDA-MB-231 cell line ABC28 that has been well characterized previously (25). Large scale immunoprecipitations of endogenously expressed PRA and PRB from ABC28 cells were carried out. The gel bands containing immunoprecipitated PR were excised and processed to tryptic peptides for LC-MS/MS analysis. Lys-183-modified peptides with a mass gain of 42.01 Da in lysine residue were consistently identified in almost all preparations. As is shown in Fig. 1, A and B, two tryptic peptides of 3ϩ charge state with monoisotopic masses at 522.620 and 536.623 Da, respectively, were detected. These two peptides have similar MS spectra but differ in mass by 42.01 Da (536.623 Ϫ 522.620) ϫ 3), suggesting that the peptide with a mass of 536.623 is modified by acetylation or trimethylation. The MS/MS spectrum of a triply charged precursor ion at m/z 522.62022 (calculated molecular mass 1567.86066 Da) of the peptide VGDSSGTAAAHKVLPR was detected at a retention time of 16.88 min (Fig. 1A). The MS/MS spectrum of a triply charged ion at m/z 536.623430 corresponding to the mass of the corresponding modified peptide (calculated molecular mass 1609.87029 Da) was identified at a later retention time, 22.17 min (Fig. 1B).
The precursor ions of the unmodified and modified peptides detected in the MS spectra were fragmented by MS/MS to identify the peptide and to assign the modification site. The MS/MS spectra and the fragment ion assignments were shown in Fig. 2. The fragment ions of the peptides were assigned to the b or y ion series by Mascot and confirmed by manual inspection of the MS/MS spectra. The Lys-183 is sandwiched by a series of b and y ions in Fig. 2, B and C. From the manual inspection of the doubly charged y ions series, we observed mass shifts of 42 Da in the y 2ϩ ion series of the modified peptide spectrum from y 5 2ϩ to y 15 2ϩ (Fig. 2B) when compared with the corresponding y 2ϩ ion series of the unmodified peptide ( Fig. 2A). For example, the increase in m/z value between y 5 2ϩ of the modified peptide (m/z ϭ 327.72) and y 5 2ϩ of the unmodified peptide (m/z ϭ 306.71) is 21, corresponding to a 42-Da mass increase when multiplied by its charge (ϩ2). Therefore, it could be deduced that the modification took place at Lys-183. The detailed b and y ions profiles of these two peptides from the Mascot search is provided in Mascot Peptide View in supplemental data 1 (unmodified peptide) and supplemental data 2 (modified peptide).
To further confirm Lys-183 acetylation, we analyzed FLAGtagged PRB because a larger amount of PRB can be pulled down by FLAG antibody. MDA-MB-231 cells were stably transfected with FLAG-tagged PR, and the isolated FLAG-PRB was analyzed by LC-MS/MS. The modified peptides with the mass gain of 42.01 were consistently identified with very high confidence. Fig. 2C illustrates a representative MS/MS spectrum from a doubly charged precursor ion and its fragment ion assignment to VGDSSGTAAAHK(Ac)VLPR peptide. The peptide was identified by Mascot with an ion score of 115, and manual inspection of the b ion series and an almost complete y ion series that sandwiched the Lys-183 site indicates that the positive mass shifts of 42 Da started from y 5 and extended to y 13 but were not observed from y 2 to y 4 , which confirms the presence of modification at Lys-183. For example, the mass difference between y 4 (m/z ϭ 484.43) and y 5 (m/z ϭ 654.45) of the modified peptide is 170.02 Da, which corresponds to the mass of lysine (128.17) and an additional mass of 42 Da. The manual inspection of the b ion series flanking Lys-183 also indicates that the positive mass shift of 42.01 takes place at Lys-183. The detailed b and y ion profiles of this peptide from Mascot search is provided in Mascot Peptide View in supplemental data 3.
The peptide VGDSSGTAAAHK(Ac)VLPR was also detected in endogenously expressed PR in breast cancer cell line T47D. Manual inspection of the y ions series also confirmed the site of the 42-Da mass shift to be at Lys-183 (supplemental data 4 and 5). The detailed b and y ion profiles of the peptides from Mascot search are provided in Mascot Peptide View in supplemental data 6 (unmodified) and 7 (modified).
The observed mass shift of 42 Da in precursor and fragments ions could be attributable to Lys-183 acetylation (42.0106 Da) or trimethylation (42.0470 Da). Because the LTQ-FT Ultra instrument provides high resolution and mass accuracy with mass error of Ͻ10 ppm, the Lys-183 modification is positively identified as acetylation based on the accurate detection of the mass difference of 42.01 Da in modified and unmodified precursor ions.
The unambiguous identification of Lys-183 as acetylation but not trimethylation is further supported by the charge states detected in the non-acetylated and acetylated peptides. The non-acetylated VGDSSGTAAAHKVLPR peptide was detected in 3ϩ and 4ϩ charge states, whereas the acetylated VGDSSG-TAAAHK(Ac)VLPR peptide was detected in 2ϩ and 3ϩ charge states. This is consistent with the fact that acetylation removes the protonation site at lysine, but trimethylation does not. Moreover, acetylation at lysine increases the hydrophobicity of the peptide due to loss of the protonation site at Lys-183, resulting in a significant increase in the peptide retention time from 16.88 min (unmodified) to 22.17 min (acetylated) in the reverse phase C18 column during LC-MS/MS analysis.
Verification of Lys-183 Acetylation by Acetyl-lysine Antibody-PR acetylation at Lys-183 was further verified with a pan-acetyllysine antibody (Fig. 3). WT PRB or mutant K183R was transiently transfected into COS7 cells. Immunoprecipitated PR was analyzed for acetylation by Western blotting analysis. Acetylation of PRB was undetectable in the absence of ligand. Consistent with the observations by Daniel et al. (8), PR acetylation is increased following treatment with progestin R5020 or trichostatin A (TSA), a histone deacetylase (HDAC) inhibitor. Combined treatment of TSA and R5020 resulted in greater induction of PR acetylation than either treatment alone. More importantly, PR acetylation was not detectable in K183R mutant under all treatments, indicating that Lys-183 is the major site of acetylation on PR.
PR Is Acetylated at Lys-183 by p300 and CBP by in Vitro Acetylation Assay-Acetylation of steroid receptors has been shown to be catalyzed by histone acetyltransferases. Several acetyltransferases, such as p300, CBP, and PCAF, have been shown to acetylate nuclear receptors and modulate their activities (31). To identify the enzyme that acetylates PR at Lys-183, we conducted an in vitro acetylation assay with the potential acetyltransferases (recombinant FLAG-p300 or immunoprecipitated HA-CBP and FLAG-PCAF). It was found that all three enzymes could acetylate full-length PRB (Fig. 4, A-C). However, because PCAF is associated with p300/CBP, it is not clear if the activity comes from PCAF itself or the associated proteins.
We next asked if these enzymes could specifically acetylate Lys-183 of PR because Lys-183 is not contained in the typical acetylation consensus sequence (K/R)XKK. The peptide acetylation assay showed that both recombinant p300 and HA-CBP acetylated Lys-183, whereas the substitution of the residue Lys-183 with glutamine abolished acetylation (Fig. 4, D and E). On  The PR peptide sequences are KVGDSSGTAAAHK 183 VLPRGLSPARQL (wild type) and KVGDSSGTAAAHQ 183 VLPRGLSPARQL (K183Q replacement). Recombinant histone H3 protein was used as a positive control. Products were resolved by SDS-PAGE, and the acetylated peptide was detected by autoradiography. G, in vivo PR acetylation by p300. COS7 cells were transfected with vector pcDNA3.1 (1 g) or FLAG-tagged PRB (1 g) with or without FLAG-tagged p300 (4 g) for 48 h before they were treated with 10 nM R5020 for 1 h. Whole cell lysates were collected and immunoprecipitated (IP) with anti-FLAG antibody. The proteins resolved on Western blot were detected using the respective antibodies again as indicated. p300 increased the levels of acetylated PRB both in the presence and absence of R5020. H, abrogation of PR acetylation by p300 gene silencing. ABC28 cells were transfected with 40 nM scrambled siRNAs or p300 siRNAs for 72 h before whole cell lysates were collected for immunoprecipitation and Western blotting analysis of PR acetylation. the other hand, PCAF failed to acetylate Lys-183 of PR under the same assay conditions, although the enzyme strongly acetylated the positive control full-length recombinant histone H3 protein (Fig. 4F). This is consistent with our earlier notion that FLAG-PCAF-associated p300 or CBP could be involved in the acetylation of full-length PR, but the amount of co-immunoprecipitated p300 and CBP was insufficient to generate a detectable acetylation signal of the peptide. This is also supported by the observation that the peptide acetylation signals by p300 and CBP were also low, and hence a large amount of the enzymes would be needed to generate a detectable signal. Therefore, p300 and CBP but not PCAF can target PR for acetylation at Lys-183. However, the data cannot rule out the possibility that PCAF acetylates a previously reported acetylation motif, lysines 638 -641 on PR (8).
PR Is Acetylated at Lys-183 by p300 in Vivo-Because p300 and CBP are closely related transcriptional co-activators with extensive sequence and structural homology (32) and overlapping functions (33), we chose from here on in to focus on p300 for its role in PR acetylation and function. To confirm that Lys-183 as an authentic in vivo acetylation site by p300, we carried out an in vivo PR acetylation assay by co-expressing p300 and PRB in COS7 cells, and PR acetylation was detected by pan-acetyl-lysine antibody following co-immunoprecipitation. As is shown in Fig. 4G, PR acetylation was markedly increased by p300 overexpression, and PR acetylation by p300 was further increased in the presence of PR ligand R5020.
Having established that PR was acetylated in vitro and in vivo by p300, we next assessed whether p300 was the major acetyltransferase responsible for PR acetylation. p300 in ABC28 cells was knocked down using siRNA against p300, and its effect on PR acetylation level was assessed. After p300 knockdown, the PR protein was immunoprecipitated and visualized by Western blotting for acetylation (Fig. 4H). The transfection of p300 siRNAs resulted in undetectable levels of p300 by Western analysis while causing minimal change in PR protein levels (Fig.  4H). The silencing of p300 abrogated PR acetylation. Taken together, these data indicate that p300 is primarily responsible for PR acetylation at Lys-183.
PR Acetylation at Lys-183 Enhances PR Activity Specifically at PRE Promoter-We next tested the effect of Lys-183 acetylation on PR activity using Lys-183 mutants in a cell-based PR reporter gene assay. The luciferase reporter gene is driven by a 2ϫ canonical progesterone response element (PRE2-Luc). Following treatment with 10 nM R5020 for 12 h, cells transfected with WT PRB exhibited around 400-fold induction of PR reporter gene activity relative to vehicle (0.1% EtOH)-treated controls (Fig. 5A). In contrast, the acetylation mimic mutant, K183Q, induced the reported gene activity by 660-fold, which is significantly higher (p Ͻ 0.001) than that of wild-type PRB. On the other hand, the K183R mutant exhibited similar activity as the WT PRB.
It is known that PR can be activated by the partial agonist property of PR antagonist RU486. We tested if PR acetylation had any effects on the partial agonist activity of RU486. Consistent with the results of R5020-induced PR activity, acetylation-mimicking mutant PR-K183Q also exhibited heightened PRE transcriptional activity in response to RU486 treatment (WT RB, 5.07-fold; PRB-K183Q, 7.12-fold; PRB-K183R, 5.19-fold) (Fig.  5B). Together, these results indicate that Lys-183 acetylation heightens the transcriptional activity of PRB in response to both progestin and agonist property of anti-progestin.
To demonstrate the role of p300 acetylation of PR on the transcriptional responses of PR on PRE activity, the effect of p300 overexpression on the transcriptional activity of WT PRB, PRB-K183Q, or PRB-K183R was investigated in the PR reporter assay. p300 overexpression enhanced WT PRB transcription activity on the PRE promoter by ϳ450% (Fig. 5C). In contrast, the transcription enhancing effect of p300 on K183Q and K183R mutants was only 174 and 130%, respectively (Fig. 5C). The data suggest that p300 enhanced PRB activity predominantly via Lys-183 acetylation, and Lys-183 mutation markedly abolished the effect of p300. This notion is supported by the finding that Lys-183 is also important for HDAC inhibitor TSA to enhance PR activation. TSA preserves protein acetylation through inhibition of HDAC activity. As a result, TSA treatment led to an increase of 32% of WT PRB activity (Fig. 5D). However, this effect on PRB-K183Q or PRB-K183R was only 18 and 12%, respectively, which were significantly lower (p Ͻ 0.0001) than that on the WT PRB. These results suggest that PR acetylation at Lys-183 by p300 positively regulates PR transcriptional activity, and the effect of p300 on Lys-183 mutants is muted because the mutants were no longer acetylated by p300.
PR can regulate gene transcription through tethering with other transcription factors, including Sp-1, AP-1, and NFB. For example, PR has been shown to attenuate NFB reporter activity in a ligand-dependent manner via the protein-protein interactions of PR with the p65 subunit of NFB (34,35). We also addressed if Lys-183 acetylation by p300 regulates the activity of PR on NFB-mediated gene regulation using the well characterized 5xRel-Luc reporter gene assay. The results showed that WT PRB and Lys-183 mutants attenuated the transcriptional activity of the NFB to a similar extent (3-4fold) (Fig. 5E). Furthermore, p300 overexpression had no effect on PR activity in attenuating NFB activity. Western blotting analysis showed similar protein expression of Lys-183 mutants as compared with WT PRB (Fig. 5F). Thus, PR acetylation by p300 at Lys-183 specifically regulates PR activity on its direct target genes, whereas PR acetylation does not influence PR tethering with NFB.

Lys-183 Acetylation Positively Regulates the Expression of PRE-containing Target Genes but Has Minimal Effect on PR trans-Repression on NFB Target Genes in Breast Cancer Cells-
Data obtained with a reporter gene assay showed that PR acetylation at Lys-183 by p300 promotes PR-mediated transactivation on PRE-driven gene reporter but has no effect on the NFB reporter gene. We then asked if the same mechanism of regulation occurs with endogenous genes in the PR-transfected MDA-MB-231 cell line ABC28. We did this by determining if p300 gene silencing could attenuate specifically PRE-containing gene expression. ABC28 cells were transiently transfected with negative control siRNAs (scrambled siRNA) or two different p300 siRNAs, which reduced p300 mRNA expression by 60 -80% (Fig. 6A). Western blotting analysis showed that both p300 siRNAs also reduced the protein levels of p300 by at least 70% (Fig. 6C). We also verified that PR mRNA (Fig. 6B) and protein levels (Fig. 6C) were not significantly reduced by p300 siRNA as compared with the control siRNA. Furthermore, ligand-induced PR protein band upshift as a result of PR phosphorylation occurs normally following p300 gene silencing.
PR Acetylation by p300 Accelerates PR-PRE Binding Kinetics-Like other members of the nuclear receptor family, PR regulates gene transcription through binding to specific gene sequence and recruiting transcription co-regulators to the gene promoter (41). Upon ligand binding, PR recruits SRC-1, which in turn recruits p300/CBP to the gene promoter. To understand the mechanisms by which PR acetylation by p300 enhances specifically PR transcriptional activity on its direct target genes, we tested the hypothesis that Lys-183 acetylation enhances the rate or duration of PR-DNA binding. ChIP assays were carried out to monitor the influence of PR acetylation on the recruitment of PR to the well characterized intronic PRE on the promoter of FKBP5. Fig. 7A shows that p300 gene silencing resulted in a decrease of PR recruited to FKBP5 PRE. Treatment of TSA (100 nM) increased ligand-induced PR recruitment to the FKBP5 promoter (Fig. 7B). More importantly, TSA treatment is associated with accelerated PR binding to the canonical  5 g) and Renilla (1 ng) reporters. The PR-Luc activities were analyzed under various conditions. A, PR acetylation mimic PRB-K183Q induced higher PRE transactivation activity in response to R5020. B, PR acetylation mimic PRB-K183Q induced higher PRE transactivation activity in response to Ru486. C, p300 co-activation of PR is dependent on Lys-183. HeLa cells were transfected with plasmids as described in A in addition to 50 ng of PCI-FLAG p300 or PCI vector control. The increase of PRB-K183R or PRB-K183Q activity in response to p300 is only one-third of that of WT PRB. D, the increases of PRB-K183R and PRB-K183Q activity in response to HDAC inhibitor TSA are 50% or less than that of PRB. Following transfection as in A, HeLa cells were treated with 100 nM TSA or vehicle control in the absence or presence of 10 nM R5020 for 1 h before analysis for PRE-Luc activity. E, PR acetylation mutants exhibit similar inhibitory effects on NFB activity as WT PRB. HeLa cells were transfected with 5 ng of various PRB constructs, NF-B reporter 5xRel-Luc (1.5 g), and Renilla (1 ng) reporters in the presence of PCI-FLAG p300 or PCI vector control (50 ng). Cells were then treated and analyzed as in A. Asterisks denote statistical significance (****, p Ͻ 0.0001), whereas n.s. denotes non-significant change determined by unpaired Student's t tests. F, relative protein expression of WT PRB-, PRB-K183Q-, and PRB-K183R-transfected cells. ␤-Actin was detected as the loading control. Error bars, S.E. PRE on the FKBP5 gene. As is shown in Fig. 7B, there is a timedependent increase of PRE binding following R5020 treatment both in the absence and presence of TSA. At every time point, more PR was recruited to the PRE in the presence of TSA. Moreover, PRE binding with TSA treatment was detected at an earlier time point than that without TSA treatment. Clearly, TSA-treated sample after 10-min R5020 treatment shows more PRE binding than that without TSA at 30 min. These observations suggest that PR acetylation not only increases but also accelerates its DNA binding.
To evaluate the specific involvement of p300 acetylation of Lys-183 in the PR-PRE binding, we compared the PRE binding between WT PRB and PRB-K183R in the presence and absence of p300 overexpression in a time course experiment (Fig. 7C). Similar to the effect of TSA treatment on PR-PRE recruitment, p300 overexpression is associated with increased and accelerated WT PRB binding to the PRE sequences on the reporter plasmid. In contrast, p300 overexpression had no effect on PRB-K183R binding to PRE at all of the time points tested. This suggests that the effect of p300 overexpression on increased DNA binding was mediated by Lys-183 acetylation.
Because TSA treatment and p300 overexpression enabled PRB to associate with PRE at an earlier time, we compared the PRE binding kinetics of WT PRB with that of acetylation-mimicking mutant PRB-K183Q. Plasmid immunoprecipitation assays coupled with quantitative real-time PCR were carried out to measure PR binding to the PRE-Luc vector. The assay allows us to compare the PRE binding kinetics between WT PRB and acetylation mimic mutant PRB-K183Q with multiple samples in transient transfection experiment. First, we confirmed using duplication samples that PRB-K183Q pulled down the canonical 2XPRE-Luc sequence more than WT PRB both in the absence and presence of R5020 (Fig. 7D). The magnitude of increase in DNA binding for PRB-K183Q as compared with WT PRB was ϳ30 -40%, which is similar to its increase of transcriptional activity in PRE-luciferase assays and the increased recruitment to PRE with p300 overexpression. The ligand-independent binding is probably responsible for the ligand-independent activity detected in the PRE-Luc assays. Next, we compared their PRE-Luc binding kinetics in 5-min intervals over a 45-min period. It appears that K183Q mutant was more rapidly recruited to the PRE sequences following R5020 treatment (Fig. 7E). More interestingly, K183Q binding exhibited a cyclic fluctuation every 20 min on the synthetic PRE promoter. It reached peak promoter occupancy after 10 min of hormone treatment and returned to base line after 20 min FIGURE 6. p300 siRNA reduced R5020-induced expression of direct PR target genes, whereas it had minimal effect on PR trans-repression of NFB target genes in ABC28 cells. ABC28 cells were transfected with NC or p300 siRNAs (40 nM) for 72 h before they were treated with or without 10 nM R5020 for 3 h. The cells were then harvested for RNA and protein analysis. A, p300 expression was reduced by p300 siRNA1 and siRNA2 by 60 and 80%, respectively, relative to scrambled siRNA control. B, PR mRNA levels were not affected by p300 siRNA transfection. C, Western blotting analyses of p300 and PR proteins following p300 siRNA treatment. ␤-Actin was probed as loading control. D-F, mRNA expression of FKBP5 (D), 11␤-HSD2 (E), and MUC1 (F) in p300 siRNA 1 and 2-transfected ABC28 cells were significantly reduced in response to R5020 treatment. G-I, R5020-induced suppression of CSF2 (G), IER3 (H), and IL-6 (I) in p300 siRNA-transfected ABC28 cells was not significantly affected. Statistical significance was determined using Student's unpaired t test, and asterisks denote statistical significance (ϮS.E.; *, p Ͻ 0.05; ***, p Ͻ 0.001; ****, p Ͻ 0.0001), whereas n.s. denotes non-significant change as determined by unpaired Student's t tests. Error bars, S.E.
before the next cycle. In contrast, WT PRB binding increased slowly over the period tested and had yet to reach peak promoter occupancy by 45 min. The cyclic fluctuations in the promoter binding of nuclear receptors and its co-regulators are well reported phenomena (29,42). These data suggest that acetylation mimic K183Q mutant assembles onto the PRE promoter at a faster rate and renews the assembly more quickly. Thus, the acetylation of PR by p300 could enhance the kinetics of its occupancy on the promoter.
PR Acetylation Is Associated with Increased PR Phosphorylation at Ser-294-Lys-183 is located in NTD, on which more than a dozen phosphorylation sites are situated. It was reported that mutation of lysines at the KFKK (amino acids 638 -641) acetylation motif delayed PR phosphorylation at Ser-294, Ser-345, and Ser-400. Among these, Ser-294 phosphorylation is the most studied phosphorylation site on NTD and is critical for PR activity (43,44). We asked the question of whether there is any functional interplay between Lys-183 acetylation and Ser-294 phosphorylation by testing if the increase of the Lys-183 acetylation level by HDAC inhibitor TSA could increase the levels of Ser-294 phosphorylation. Expectedly, TSA treatment increased acetylated PRB levels compared with untreated controls (Fig.  8A). This was associated with corresponding increases of Ser-294 phosphorylation at both time points after R5020 treatment. It also appears that Ser-294 phosphorylation occurred earlier in response to TSA treatment. Sample treated with TSA presents a prominent band at 15 min after R5020 treatment. At the same FIGURE 7. PR acetylation at 183 accelerates PR-PRE binding kinetics. A, p300 silencing reduces PR recruitment to the FKBP5 promoter. ABC28 cells were treated with vehicle or 10 nM R5020 for 15 min. Fixed DNA-protein complex was immunoprecipitated with PR antibody H190 or rabbit IgG control. Relative levels of PR-PRE promoter interaction were measured by PCR in duplicates, and 1% DNA input was included as a loading control. B, HDAC inhibitor TSA accelerates the recruitment of PR to FKBP5 PRE. ABC28 cells were treated with R5020 according to the time points indicated in the figure, and ChIP assays were performed as described in A. C, accelerated recruitment of PRB to PRE-Luc by p300 is dependent on Lys-183. HeLa cells were transfected with 10 ng of pcDNA3.1 vector, WT PRB, or PRB-K183R in addition to 1.5 g of PRE2-TATA-luciferase vector and 100 ng of PCI-FLAG p300 or PCI vector control. Cells were then treated and analyzed for PR-PRE binding according to the time points indicated in the figure. Relative levels of PR-PRE promoter interaction were measured by PCR, and 1% DNA input was included as a loading control. D, PRB-K183Q shows increased binding to PRE-Luc vector by plasmid immunoprecipitation assay as described in C. Relative levels of PR-PRE promoter interaction were measured as described in C in duplicates. E, PRB-K183Q exhibits faster PRE binding kinetics. The plasmid immunoprecipitation assay was carried out as described in C according to the time points indicated in the figure. Immunoprecipitated plasmid DNA is quantified by real-time PCR. The results are expressed as relative binding of PR-PRE following normalization against 1% DNA input control (mean Ϯ S.E. (error bars)).

FIGURE 8. Acetylation of PRB is associated with increased PR phosphorylation.
A, the stabilization of acetylated PR by TSA enhances its phosphorylation at Ser-294. COS7 cells were transiently transfected with FLAG-tagged PRB. Cells were serum-starved for 24 h and treated with TSA as described in the legend to Fig. 3, followed by R5020 treatment for different time points (indicated in the figure) before collection for PR immunoprecipitation. Proteins resolved on Western blot were detected with pan-acetyl-lysine, PR, and phospho-Ser-294 antibodies. B, in vivo acetylation of PR by p300 increases PR phosphorylation. COS7 cells were transiently transfected with FLAG-tagged PRB in addition to vector control or FLAG-tagged p300 (4 g). Cells then treated with 10 nM R5020 for different time points indicated in the figure. Proteins were detected using the respective antibodies. C, acetylation mimic mutant PRB-K183Q shows higher levels of Ser-294 phosphorylation than WT PRB or PRB-K183R in response to various R5020 dosages (10 Ϫ9 , 10 Ϫ8 , or 10 Ϫ7 M). Western blotting analysis was carried out to detect PR and PR phosphorylation at Ser-294 using the respective antibodies. GADPH was probed as a loading control. time point, sample without TSA treatment showed no detectable Ser-294 phosphorylation (Fig. 8A). Similarly, overexpression of p300, which elevated the levels of acetylated PR with or without R5020 treatment in a time-dependent manner, resulted in time-dependent increases of phosphorylation at Ser-294 as compared with cells with basal p300 expression (Fig.  8B).
To further characterize the specific effects of Lys-183 acetylation on PR phosphorylation, we compared Ser-294 phosphorylation among WT PRB, PRB-K183Q, and PRB-K183R following transient transfection in COS7 cells. As is shown in Fig. 8C, Ser-294 phosphorylation levels increases with increasing concentration of R5020 in all three forms of PRB. However, PRB-K183Q has higher levels of phosphorylation at Ser-294 at all R5020 dosages tested as compared with WT PRB and K183R. Taken together, these findings suggest that PR acetylation at Lys-183 facilitates PR phosphorylation at Ser-294, which, in turn, may lead to greater PR activity.

DISCUSSION
To date, the identification of acetylation of steroid hormone receptors has been based on the presence of acetylation consensus motif (K/R)XKK (31). By LC-MS/MS analysis, this study reports the identification of a novel acetylation site of PR at Lys-183 that is not contained within such a consensus motif. The acetylation was detected in both the endogenously and exogenously expressed PR from breast cancer cell lines. Close inspection of the peptide sequence containing Lys-183, TAAAHK 183 VLPRG, shows that there is a positively charged Arg residue at the Lys-183 ϩ 4 position, which fits the p300 substrate preference reported (45). Indeed, p300 directly acetylates PR at Lys-183 by both in vitro and in vivo acetylation assays. Lys-183 acetylation is associated with accelerated ligand-induced PR binding to its cognate PRE sequences and heightened PR activation kinetics on direct PR target genes, highlighting a critical involvement of Lys-183 of NTD in PR PR-DNA interaction.
Our study is consistent with an earlier study that PR acetylation is ligand-induced and can be increased with deacetylase inhibitor (8). However, the study has reported that PR is acetylated at two or more lysine residues at the acetylation consensus motif 638 KXKK 641 in the hinge region (8). Mutation of all three lysines is required to abolish the acetylation detection by antibody against acetylated lysines. This is in contrast to our finding that a single mutation, K183R, diminished PR acetylation in vivo (Fig. 3), using the same pan-antibody against acetylated lysine. There may be several explanations for the discrepancies. First, although the Lys-183 mutant shows no detectable acetylation in vivo under our experimental conditions, the detection of the remaining acetylation may be limited by the assay sensitivity. Second, the three lysines ( 638 KFKK 641 ) in the hinge region may be important for PR acetylation at Lys-183; the mutation of all three abolishes Lys-183 acetylation. It is also possible that the site and level of PR acetylation are cellular context-and experimental condition-dependent. Under our experimental conditions, Lys-183 of PRB is a primary acetylation site.
PR can regulate gene expression through ligand-induced recruitment to the cognate PR binding sites, known as PRE, of the target genes (46). PR also regulates the activity of other transcription factors, such as NFB, through tethering mechanisms (35,47,48). Three lines of evidence support the notion that PR acetylation by p300 at Lys-183 specifically enhances PR activation of direct target genes with cognate PR binding sites. First, acetylation mimic mutation K183Q significantly increased progestin-induced PRE-Luc activity but had no effect on NFB reporter gene activity. Second, p300 overexpression or TSA treatment that increased the levels of Lys-183 acetylation increased markedly WT PRB-mediated PRE-Luc activity. In contrast, K183Q and K183R mutants that can no longer be acetylated are significantly less responsive to the acetylationenhancing agents. Consistently, p300 gene silencing significantly decreased progestin-induced expression of PRE-containing genes FKBP5, 11␤-HSD2, and MUC1 but had no influence on NFB target genes. This specific effect of Lys-183 acetylation on PRE-containing target genes supports the notion that Lys-183 acetylation facilitates PR-DNA interaction.
Steroid receptors are known to exhibit dynamic association/ dissociation/reassociation with their target gene promoters in a temporal manner depending on the promoter context and the presence of transcription co-regulators (29,42,49). It has been reported that p300 could potentiate PR activity by promoting the initiation and reinitiation process in PR transcription using cell-free chromatin transcription assays (13). Data presented here indicate that the effect of p300 on initiation/reinitiation process is mediated, at least in part, through Lys-183 acetylation. First, we observed that p300 gene silencing decreased PR-PRE binding (Fig. 7A), and the treatment with HDAC inhibitor TSA was associated with accelerated PR binding to the canonical PRE on the FKBP5 gene in the time point experiment (Fig.  7B). Significant binding was detected in sample treated with TSA after 5 min of progestin treatment. This is in contrast to the lack of detectable binding signal in sample without TSA treatment. Second, a PRE-Luc plasmid immunoprecipitation assay showed that acetylation mimic mutant K183Q displayed more rapid PR-PRE binding kinetics in response to progestin (Fig. 7E). When PRE binding was measured in 5-min intervals over a 45-min period, PRB-K183Q binding exhibited a cyclic fluctuation every 20 min on the synthetic PRE promoter. On the other hand, WT PRB binding to PRE has yet to reach peak promoter occupancy by 45 min, which is consistent with the average cycling time of 60 -75 min reported for PR and estrogen receptor ␣ (29,42). These data suggest that PRB-K183Q is recruited onto the PRE promoter at a faster rate (faster initiation) and renews the assembly more quickly (reinitiation), leading to greater transcriptional outcomes. It has been reported that CBP/p300 can recognize and bind acetylated lysine residues in histones and transcription factors through their bromodomains (50 -53). It is plausible that p300 acetylates Lys-183 of PR to create a docking site for a better grip or more efficient recruitment of general transcription machinery. An increase of Lys-183 acetylation by p300 can thus serve to heighten PR activity in response to cellular cues.
Phosphorylation of PR has been shown to be a pivotal regulator of the transcriptional response to progestin (44, 54 -56).
Ser-294 phosphorylation is one of the most important PR phosphorylations. It is involved in regulating multiple aspects of PR activity, including nucleocytoplasmic shuttling, protein ubiquitination, and PR activation (57). For example, phosphomimic mutation by replacement of Ser-294 with aspartic acid (S294D) created hyperactive PR, whereas S294A mutant is hypoactive (58). Interestingly, the heightened activity of acetylated PR at Lys-183 is associated with increased levels of PR phosphorylation at Ser-294 (Fig. 8). p300 overexpression and TSA treatment both elevated Lys-183 acetylation, resulting in evident increases of Ser-294 phosphorylation in a time-dependent manner. More specifically, the Lys-183 acetylation mimic, PRB-K183Q, exhibits higher levels of phosphorylation at Ser-294 than WT PRB and K183R. It is conceivable that increased Ser-294 phosphorylation in association with Lys-183 acetylation plays a part in acetylation-induced increase of PR activity.
Past studies have reported both negative and positive interplays between acetylation and phosphorylation. Acetylation of STAT1 negatively regulates interferon-induced STAT1 phosphorylation by recruiting tyrosine phosphatase TCP45 (59). On the other hand, p53 acetylation at Lys-373 leads to its hyperphosphorylation, and this allows better binding of p53 with promoters with which p53 normally interacts with low affinity (60). Note that in the present study, the detection of earlier and higher Ser-294 phosphorylation in association with Lys-183 acetylation also coincides with a faster DNA binding kinetics and greater amount of DNA binding. Because Ser-294 phosphorylation is a positive regulator of PR transcription, higher levels of phosphorylation at 294 in acetylated PR probably drive enhanced PR-DNA binding dynamics.
Combinations of different modifications have been proposed to serve as a "code" in regulating diverse function of proteins. In p53, different acetylation sites have differential effects on its target gene expression patterns via influencing p53 phosphorylation at different sites (60). Our study suggests that the combination of PR post-translational modifications, such as acetylation and phosphorylation, also presents an attractive regulatory mechanism for fine tuning the control of PR target genes. It is likely that interplays among the modifications in different combinations add dimension to the gene regulation strategy in nature that allow the same protein to exert diverse functions in different tissues (e.g. mammary gland and uterus) and under various physiological conditions.