Phosphorylation of SOX9 by Cyclic AMP-Dependent Protein Kinase A Enhances SOX9's Ability To Transactivate a Col2a1 Chondrocyte-Specific Enhancer

doi:10.1128/MCB.20.11.4149-4158.2000

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Molecular and Cellular Biology, June 2000, p. 4149-4158, Vol. 20, No. 11
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Phosphorylation of SOX9 by Cyclic AMP-Dependent Protein Kinase A Enhances SOX9's Ability To Transactivate a Col2a1 Chondrocyte-Specific Enhancer

Wendong Huang, Xin Zhou, Véronique Lefebvre, and Benoit de Crombrugghe^*

Department of Molecular Genetics, The University of Texas M. D. Anderson Cancer Center, Houston, Texas 77030

Received 3 February 2000/Returned for modification 2 March 2000/Accepted 6 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Sox9 is a high-mobility-group domain-containing transcription factor required for chondrocyte differentiation and cartilageformation. We used a yeast two-hybrid method based on Son of Sevenless(SOS) recruitment to screen a chondrocyte cDNA library and foundthat the catalytic subunit of cyclic AMP (cAMP)-dependent proteinkinase A (PKA-C $alpha$ ) interacted specifically with SOX9. Next we foundthat two consensus PKA phosphorylation sites within SOX9 couldbe phosphorylated by PKA in vitro and that SOX9 could be phosphorylatedby PKA-C $alpha$ in vivo. In COS-7 cells cotransfected with PKA-C $alpha$ andSOX9 expression plasmids, PKA enhanced the phosphorylation ofwild-type SOX9 but did not affect phosphorylation of a SOX9 proteinin which the two PKA phosphorylation sites (S₆₄ and S₂₁₁) weremutated. Using a phosphospecific antibody that specifically recognizedSOX9 phosphorylated at serine 211, one of the two PKA phosphorylationsites, we demonstrated that addition of cAMP to chondrocytes stronglyincreased the phosphorylation of endogenous Sox9. In addition,immunohistochemistry of mouse embryo hind legs showed that Sox9phosphorylated at serine 211 was principally localized in theprehypertrophic zone of the growth plate, corresponding to themajor site of expression of the parathyroid hormone-related peptide(PTHrP) receptor. Since cAMP has previously been shown to effectivelyincrease the mRNA levels of Col2a1 and other specific markersof chondrocyte differentiation in culture, we then asked whetherPKA phosphorylation could modulate the activity of SOX9. Additionof 8-bromo-cAMP to chondrocytes in culture increased the activityof a transiently transfected SOX9-dependent 48-bp Col2a1 chondrocyte-specificenhancer; similarly, cotransfection of PKA-C $alpha$ increased the activityof this enhancer. Mutations of the two PKA phosphorylation consensussites of SOX9 markedly decreased the PKA-C $alpha$ activation of thisenhancer by SOX9. PKA phosphorylation and the mutations in theconsensus PKA phosphorylation sites of SOX9 did not alter itsnuclear localization. In vitro phosphorylation of SOX9 by PKAresulted in more efficient DNA binding. We conclude that SOX9is a target of cAMP signaling and that phosphorylation of SOX9by PKA enhances its transcriptional and DNA-binding activity.Because PTHrP signaling is mediated by cAMP, our results supportthe hypothesis that Sox9 is a target of PTHrP signaling in thegrowth plate and that the increased activity of Sox9 might mediatethe effect of PTHrP in maintaining the cells as nonhypertrophicchondrocytes.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The transcription factor SOX9 contains a high-mobility-group (HMG)-type DNA-binding domain that shows 50% identity to thatof the mammalian testis-determining factor SRY (35) and a transcriptionactivation domain located at the carboxyl terminus of the molecule(27, 31). During embryonic development, expression of Sox9parallels that of the gene for type II collagen (Col2a1) in allchondrocyte progenitors and chondrocytes (27, 36, 37). Inaddition, Sox9 is also expressed in gonadal ridges in male andfemale embryos, and later, whereas its expression is stronglydownregulated in female gonads, it is found at high levels inthe Sertoli cells of male gonads (13, 26). Sox9 is also expressedin otic vesicles and in discrete areas of the heart, kidney, andnervous system of mouse embryos (27, 37). Our recent experimentsusing mouse embryo chimeras derived from Sox9^/ embryonic stem cells demonstrated that Sox9 is required for chondrocytedifferentiation and cartilage formation (3). In contrast towild-type chondrocytes, the mutant cells had the aspect of undifferentiatedmesenchymal cells and could not express chondrocyte-specific markerssuch as Col2a1 and the genes for the $alpha$ 2 chain of type IX collagen(Col9a2), the $alpha$ 2 chain of type XI collagen (Col11a2), and aggrecan.In addition, neither cartilage nor type II collagen formed interatomas derived from Sox9^/ embryo stem cells. Thus, Sox9 has an essential role in determiningthe fate of chondrocytes. In humans, heterozygous mutations inand around the SOX9 gene cause campomelic dysplasia (CD), a lethaldisorder involving abnormalities in skeletal structures derivedfrom cartilage (8, 10, 15, 25, 33). In many cases thedisease is believed to be due to SOX9 haploinsufficiency (19,25). The skeletal anomalies in CD patients include bowing andangulation of the long bones, micrognathia, hypoplasia of thepelvis and scapulae, cleft palate, and a missing pair of ribs.Sex reversal is found in 75% of XY CD patients, which impliesthat SOX9 also functions in sex determination in humans (24,34). Sox9 binds to essential sequences in chondrocyte-specificenhancers of the Col2a1 (19) and the Col11a2 (5) genes, andforced expression of SOX9 activates these enhancers in nonchondrocyticcells. Ectopic expression of SOX9 also activates the Col2a1 genein transgenic mice (2). These experiments provided evidencethat these genes are direct targets forSox9.

Two other members of the Sox family of transcription factors, L-Sox5 and Sox6, also bind to chondrocyte-specific enhancerregions in the Col2a1 and Col11a2 genes (22). L-Sox5 and Sox6,which are highly similar to each other, are coexpressed with Sox9during chondrogenesis. In cotransfection experiments, they cooperatewith Sox9 in activating the Col2a1 gene (22). We thus hypothesizedthat L-Sox5 and Sox6 act together with Sox9 to control chondrocytedifferentiation.

In the present study, in order to identify possible SOX9-interacting proteins that could control SOX9 activity, we screeneda primary chondrocyte cDNA library using a yeast two-hybrid methodand found specific interactions between SOX9 and the catalyticsubunit of protein kinase A (PKA-C $alpha$ ). In cultured chondrocytes,cyclic AMP (cAMP) enhances the expression of several markers ofchondrocyte differentiation, such as Col2a1, link protein, andaggrecan (14, 23, 28); cAMP also mediates the effects ofthe parathyroid hormone-related peptide (PTHrP), a known modulatorof chondrocyte differentiation in growth plates (12, 29).Hence, we postulated that the interactions between SOX9 and PKA-C $alpha$ may be physiologically relevant and asked whether SOX9 might bea target for PKA phosphorylation and whether such phosphorylationmay affect the activity of SOX9. We found that SOX9 can be phosphorylatedby PKA and that this phosphorylation increases SOX9 binding toa Col2a1 enhancer element and stimulates SOX9 transcriptionalactivity. The finding that Sox9 phosphorylated at one of the twoPKA phosphorylation site was mainly localized to the prehypertrophiczone of the growth plate in vivo suggests the hypothesis thatSox9 may be a target for PTHrPsignaling.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

cDNA library construction and SRS screening. Total RNA was extracted from primary chondrocytes isolated from the ribs of newborn mice and cultured for 48 h. After polyadenylatedRNA purification, synthesis of double-stranded cDNA with randompriming and ligation of adapters were performed with the SuperscriptChoice system from Gibco-BRL (Gaithersburg, Md.). The cDNA wasdigested with EcoRI and inserted into the pYES-2 plasmid vector(1) 3' to the DNA for a v-Src myristoylation sequence, whichwas to anchor the library-derived polypeptides to the cytoplasmicmembrane. Full-length human SOX9 coding sequence was cloned inthe pADNS vector (1) in frame with and 3' to the carboxy terminusof the Son of Sevenless (SOS) cDNA sequence, with six glycinecodons inserted between the SOS and SOX9 sequences. SOS recruitmentsystem (SRS) screening was performed as described by Aronheimet al. (1) with some modifications. The cdc25-2 Saccharomycescerevisiae strain was first transformed with plasmid pADNS-SOS-SOX9and subsequently transformed with the pYES-2 cDNA library plasmids.Transformants were plated on galactose plates coated with a thinlayer of solution containing glucose (67 mg/ml). Plates were incubatedat 25°C for 2 days and at 37°C for 4 more days, after which colonieswere picked and tested for galactose-dependent growth at 37°C.Plasmids were extracted from surviving colonies and amplifiedin Escherichia coli for further retransformation into yeast cellsand DNA sequence analysis. The specificity of the interactionsbetween SOX9 and library-derived polypeptides was tested by cotransformingthe cdc25-2 cells with screening-positive cDNA library plasmidsand either empty pADNS, pADNS-p110-SOS (1), or pADNS-SOS-SOX9.

Mutagenesis and production of bacterially expressed GST-SOX9 and mutant SOX9 proteins. Serine-to-alanine substitution mutations were introduced into the two PKA phosphorylation consensus sites of SOX9 by usingthe Transformer mutagenesis kit (Clontech, Palo Alto, Calif.).The full-length SOX9 coding sequence was cloned into the pGEX4T3bacterial expression vector (Pharmacia Biotech, Piscataway, N.J.)to generate a glutathione S-transferase (GST) fusion polypeptide.The recombinant proteins were produced in bacterial strain BL21(DE3).After cell growth to an optical density at 600 nm (OD₆₀₀) of 0.6,1 mM isopropyl-1-thio- $beta$ -D-galactopyranoside (IPTG) was added toinduce protein synthesis, and cells were grown for another 4 hat 37°C. Recombinant polypeptides were purified on a GST-glutathioneaffinity column, and GST moieties were cleaved by thrombin asdescribed elsewhere (30). Purified proteins were stored at $-$ 80°C.

In vitro phosphorylation. Recombinant wild-type and mutant SOX9 proteins (100 ng) were added to a PKA reaction buffer containing 20 mM HEPES (pH 7.5),5 mM MgCl₂, 5 mM dithiothreitol, 1 mM ATP, 100 mM NaCl, and 1mM [ $gamma$ -³²P]ATP (0.5 Ci/mmol) and incubated with 50 U of PKA-C $alpha$ (Sigma)at 30°C for 30 min in a total volume of 50 µl (6). To testfor the specificity of the reaction for PKA, 1 µg of PKA inhibitor(PKI) (Sigma) was added to the reaction buffer to specificallyinhibit the activity ofPKA.

Cell culture and transfection experiments. All cell types were cultured as described previously (22). Cells were then transfected with luciferase reporter plasmidscontaining an 89-bp Col2a1 promoter without (p89Luc) or with (4x48-p89Luc)four copies of a 48-bp chondrocyte-specific Col2a1 enhancer elementand the pSV2- $beta$ -gal plasmid (an internal control for transfectionefficiency) in a ratio of 3:1 as described previously (20).All transfections were done with FuGene6 (Roche Molecular Biochemicals,Indianapolis, Ind.) according to the manufacturer's instructions.Expression plasmids for wild-type and mutant SOX9 proteins (100ng) and PKA-C $alpha$ (400 ng) were transfected as indicated in Fig.7 and 8. Luciferase and $beta$ -galactosidase activities were assayedin cell lysates prepared as described previously (20). 8-Bromo-cAMP(1 mM) and 10 or 20 µM H8 (PKA inhibitor) were added 4 h aftertransfection, and the cells were incubated for 8 h before beinglysed. Reporter activities are reported as the average of triplicatecultures in one of several representative experiments as previouslydescribed (20).

In vivo phosphorylation and immunoprecipitations. RCS cells grown in monolayer culture for 2 days were labeled with [³²P]orthophosphate (0.5 mCi/ml) for 4 h and then collected in phosphate-bufferedsaline (PBS) containing 0.5% NP-40 and 1% sodium dodecyl sulfate(SDS). COS-7 cells were cotransfected with expression plasmidsfor wild-type and m1+2 mutant SOX9 and PKA-C $alpha$ for 8 h as indicatedin Fig. 5. Cells were then labeled with [³²P]orthophosphate for 4 h and collected. Next, 25 µl of the celllysates was incubated with 15 µl of SOX9 antibody (22) or 15µl of SOX9 preimmune antiserum under gentle agitation at 4°C for2 h. A 2.5-µl volume of protein A-Sepharose beads (Sigma) wasadded and incubated for another 2 h at 4°C. The beads were washedthree times with 1 ml of buffer A (0.5% NP-40 in PBS), resuspendedin 10 µl of SDS-polyacrylamide gel electrophoresis (PAGE) sampleloading buffer, and boiled for 2 min. Half the volume of eachsample was resolved by electrophoresis on an SDS-10% polyacrylamidegel, and the gel was dried and autoradiographed. The other halvesof the samples were used for Western blotting to visualize theamount of SOX9 that wasimmunoprecipitated.

Immunofluorescence. COS-7 cells were cotransfected with plasmids expressing wild-type or mutant SOX9 and PKA-C $alpha$ or empty vector. Twenty-four hoursafter transfection, the cell monolayers were fixed with methanolfor 10 min and incubated with blocking buffer (PBS with 5% goatserum and 3% bovine serum albumin) for 30 min. SOX9 rabbit antibody(diluted 1:500 with blocking buffer) was added, and the mixturewas incubated for 1 h at room temperature. A secondary antibody(Jackson Immunoresearch, West Grove, Pa.) consisting of goat fluorescein-conjugatedanti-rabbit immunoglobulin G (diluted 1:200 in blocking buffer)was added, and the mixture was incubated for another 1 h. Cellswere then washed three times with cold PBS, the last time supplementedwith 5 µg of the DNA dye 4',6-diamidino-2 phenylindole (DAPI;Sigma) per ml. Slides were mounted with Aqua-Poly Mount (PolyScience,Warrington, Pa.).

Western blotting. Cell lysates were prepared and separated by electrophoresis on SDS-10% polyacrylamide gels as described previously (20).Western blotting was done with the enhanced chemiluminescenceECL kit from Amersham (Piscataway, N.J.). SOX9 antibodies wereused at a 1:1,000 dilution. To reprobe the membrane with anotherantibody, the previous antibodies were stripped off and the blotswere reprobed with a newantibody.

EMSAs. For electrophoretic mobility shift assays (EMSAs), the preparation of the 18-bp Col2a1 enhancer probe and the compositionof the EMSA incubation buffer were described previously (20).Full-length SOX9 or m1+2 mutant SOX9 made in E. coli (100 ng)was phosphorylated with 50 U of PKA-C $alpha$ in a volume of 50 µl. Afterphosphorylation, the proteins were incubated with the 18-bp probein the presence of 1 µg of poly(dG-dC) · poly(dG-dC) and 25 µgof bovine serum albumin at room temperature for 30 min. Unlabeled18-bp probe was added in 100-fold excess compared with the labeledprobe. The samples were then fractionated by electrophoresis througha nondenaturing 5% polyacrylamide gel in 0.5× Tris-borate-EDTAat 150 V for 3 h, and the gel was used forautoradiography.

Generation of SOX9.P antibody. A phosphopeptide derived from the SOX9 sequence in which serine 211 was phosphorylated (CYQPRRRKS₂₁₁VKNGQA) was used to immunizerabbits (Quality Controlled Biochemical, Hopkinton, Mass.). Serumfrom the rabbits was preadsorbed on an affinity column containingthe nonphosphorylated peptide to remove antibodies that were notphosphospecific and then affinity purified through a phosphopeptidecolumn. The final yield of phosphospecific SOX9 antibody (SOX9.P)was about 0.5 mg/ml.

Immunohistochemical analysis. Mouse embryo hind legs (16.5 days postcoitum) were fixed in 4% paraformaldehyde in PBS for 16 h. After dehydration, tissueswere embedded in paraffin and sectioned. Immunohistochemical stainingwas done with the DAKO EnVision+ system (Dako Corp, Carpinteria,Calif.). After rehydration, the slides were incubated in 3% hydrogenperoxide in methanol for 15 min at room temperature. Sectionswere then digested with 1% hyaluronidase for 45 min at 37°C andsubsequently heat treated at 95 to 99°C in citrate buffer (10mM, pH 6). Sections were incubated for 45 min at room temperaturewith either SOX9 or SOX9.P antibodies at a dilution of 1:30, thenwith the peroxidase-labeled polymer for 30 min, and subsequentlywith the substrate chromogen for 30 min at room temperature. Afterbeing washed with PBS, slides were mounted with the Crystal Mountaqueous mounting medium (Biomeda Corp., Foster City, Calif.).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

PKA-C $alpha$ interacts with SOX9 in a yeast two-hybrid assay. To identify proteins that interact with Sox9 in chondrocytes, we used a yeast two-hybrid method based on the Son of Sevenlessrecruitment system, called SRS (1), and screened a primarychondrocyte cDNA library using full-length SOX9 as the bait. Inthis system, interactions between a bait polypeptide fused toSOS and a cDNA-derived prey polypeptide anchored to the membranesuppress the temperature-sensitive phenotype of an S. cerevisiaecdc-25 mutant grown on galactose. For this screen, we generateda recombinant SOS-SOX9 fusion polypeptide consisting of SOS atthe amino terminus followed by a linker of six glycine residuesand the SOX9 sequence at the carboxyl terminus (Fig. 1A). Thelinker was used to avoid possible conformational interferencebetween the two protein moieties. Among 20 positive clones, 2independent cDNAs were identified as coding for PKA-C $alpha$ ; one ofthem encoded the full-length sequence of this polypeptide. Toassess specificity, yeast cells containing either an empty baitvector, a nonrelevant bait (p110-SOS) (1), or the originalbait (SOS-SOX9) were transformed together with the cDNA for full-lengthPKA-C $alpha$ , grown at 25°C, replicated on galactose and glucose plates,and incubated at 37°C (Fig. 1B). Suppression of the cdc25-2 temperature-sensitivephenotype occurred only in cells that expressed the SOS-SOX9 fusionpolypeptide and PKA-C $alpha$ on galactose plates. These results indicatedthat PKA-C $alpha$ specifically interacts with SOX9 in the yeast SRSsystem.

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FIG. 1. PKA-C $alpha$ interacts with SOX9 in yeast cells. (A) Bait plasmid used in the SRS screening. The full-length coding sequence of SOX9 was cloned into pADNS in frame with and carboxy-terminal to the SOS coding sequence. Six glycine residues were inserted between the SOX9 and SOS sequences. (B) Complementarity of the cdc25-2 temperature-sensitive mutation through specific interactions of SOX9 with PKA-C $alpha$ . The plasmid isolated from a yeast colony, which was positive upon primary library screening and encoded PKA-C $alpha$ , was retransformed into the cdc25-2 mutant strain together with either empty pADNS, pADNS-p110-SOS, or pADNS-SOS-SOX9. Four independent colonies were isolated for each plasmid combination, grown at 25°C, replica plated onto galactose and glucose (control) plates, and grown at 37°C. Only the colonies that expressed SOS-SOX9 and PKA-C $alpha$ grew on the galactose plates.

Two PKA phosphorylation consensus sites are present in the SOX9 protein sequence. The amino acid sequence R/K R/K N S/T is the consensus PKA recognition site, and either S or T is the phosphorylation site(4). Two putative PKA phosphorylation sites containing serine64 (S₆₄) and serine 211 (S₂₁₁) are present in the human SOX9 sequence,one on each side of the HMG DNA-binding domain (Fig. 2A). Thesetwo PKA recognition sites are conserved in mouse and chicken Sox9.To test the role of PKA phosphorylation in SOX9 function, we introducedserine-to-alanine substitution mutations in these two sites ofthe SOX9 sequence to generate the SOX9 mutants m1 (S64A), m2 (S211A),and m1+2 (S64A and S211A) (Fig. 2B).

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FIG. 2. Mutations of the two PKA phosphorylation sites of SOX9. (A) The amino acid sequence of human SOX9 is shown from amino acids 56 to 216, with the HMG domain highlighted in bold and the two PKA phosphorylation consensus sites shown in boxes. (B) Serine 64 and serine 211 in the PKA phosphorylation consensus sites were replaced with alanine in SOX9 mutant m1 and SOX9 mutant m2, respectively. SOX9 mutant m1+2 contained alanine substitutions at both sites.

SOX9 is phosphorylated in vitro by PKA. GST fusion polypeptides, with either the wild-type SOX9 or the m1+2 SOX9 mutant, were generated in E. coli and purified byglutathione affinity chromatography. The purified proteins weredigested with thrombin to remove the GST moiety and incubatedwith PKA-C $alpha$ and [ $gamma$ -³²P]ATP. Incubation of wild-type SOX9 resulted in the appearanceof a ³²P-labeled species of 68 kDa (the expected apparent molecular massof SOX9), the amount of which increased over time (Fig. 3A). Thisphosphorylation was completely inhibited by PKI, a specific inhibitorof PKA (Fig. 3B). With a mutant SOX9 in which the two consensusPKA phosphorylation sites were mutated (m1+2), phosphorylationby PKA was virtually abolished (Fig. 3B), although a Western blotshowed that the same amounts of SOX9 protein were present in thereactions containing wild-type and mutant SOX9. Incubation ofeither mutant m1 or mutant m2 with PKA and [ $gamma$ -³²P]ATP resulted in phosphorylation of SOX9 (data not shown), indicatingthat each site can be phosphorylated by PKA. These results alsoindicated that the two consensus phosphorylation sites of SOX9are the only sites to be phosphorylated by PKA in vitro.

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FIG. 3. Phosphorylation of SOX9 by PKA in vitro. (A) Time course. Bacterially expressed SOX9 was incubated with PKA-C $alpha$ in the presence of [ $gamma$ -³²P]ATP for 0 to 30 min, as indicated, before PKI was added to terminate the reactions. Reaction mixtures were separated by SDS-PAGE, and the gels were autoradiographed. A time-dependent increase in phosphorylated protein was obtained at the characteristic migration level of SOX9. Two faster-migrating products of PKA-C $alpha$ phosphorylation were detected that presumably correspond to incomplete or degraded recombinant SOX9 polypeptides (not shown). (B) Specific phosphorylation of sites 1 and 2. Bacterially expressed wild-type (wt) or double-mutant (m1+2) SOX9 proteins were incubated with (+) or without ( $-$ ) PKA-C $alpha$ and PKI for 30 min, as indicated above the lanes. Phosphorylation of SOX9 was determined as described for panel A. A Western blot of wild-type and m1+2 mutant SOX9 proteins shows that the same amount of each SOX9 protein species was present in all reactions.

SOX9 is phosphorylated by PKA-C $alpha$ in intact cells. To determine whether SOX9 is phosphorylated in intact cells, we labeled with [³²P]orthophosphate a well-differentiated rat chondrosarcoma cellline (RCS) that contains high levels of Sox9 protein and immunoprecipitatedSox9 with SOX9-specific antibodies from cell lysates. A single68-kDa, ³²P-labeled protein with a gel electrophoretic mobility correspondingto that of Sox9 was immunoprecipitated from RCS cell lysates (Fig.4A), whereas no corresponding signal was observed when preimmuneantiserum was used. Thus, phosphorylated Sox9 can be detectedin intact cells.

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FIG. 4. Phosphorylation of Sox9 in intact cells. (A) Endogenous Sox9 is phosphorylated in RCS cells. RCS cells in culture were incubated with ³²P-labeled inorganic phosphate for 4 h. Sox9 was immunoprecipitated from cell lysates with SOX9 antibody (Ab) and visualized by autoradiography after SDS-PAGE (lane SOX9 Ab). A unique ³²P-labeled band migrated with the characteristic 68-kDa molecular mass of SOX9. The specificity of the immunoprecipitation was assessed with SOX9 preimmune (Pre-immu.) serum. (B) PKA-C $alpha$ phosphorylates SOX9 at sites 1 and 2 in COS-7 cells. COS-7 cells were transfected with plasmids expressing wild-type SOX9 (wt), double-mutant SOX9 (m1+2), and PKA-C $alpha$ , as indicated. Cells were incubated with ³²P, and lysates were immunoprecipitated with SOX9 antibody. Autoradiographs of phosphorylated SOX9 proteins recovered after immunoprecipitation and SDS-PAGE are shown in the top panel. PKA increased the level of phosphorylation of wild-type SOX9 but not that of m1+2 mutant SOX9. A Western blot showing the amount of SOX9 protein in each sample after immunoprecipitation is presented in the bottom panel.

To determine whether PKA could phosphorylate SOX9 in intact cells, we cotransfected plasmids expressing either wild-type SOX9or the m1+2 SOX9 mutant together with a PKA-C $alpha$ expression plasmidinto COS-7 cells, which do not contain endogenous Sox9, labeledthe cells with [³²P]orthophosphate, and immunoprecipitated SOX9 from cell lysateswith a SOX9-specific antibody. In intact COS-7 cells, phosphorylationof wild-type SOX9 was increased by cotransfection with PKA-C $alpha$ (Fig. 4B). The m1+2 mutant SOX9 was phosphorylated in COS-7 cells,although to a lesser degree than wild-type SOX9, but cotransfectionwith PKA-C $alpha$ failed to increase phosphorylation of the mutant SOX9.This finding suggests that SOX9 contains other sites that canbe phosphorylated by kinases other than PKA. In summary, theseresults indicated that SOX9 is a phosphoprotein and a target forPKA phosphorylation in intactcells.

Phosphorylation does not affect the subcellular localization of SOX9. The PKA phosphorylation site containing serine 211 is included in a nuclear localization signal in the sequence PRRRKS₂₁₁(32). To determine whether PKA phosphorylation might changethe subcellular localization of SOX9 and whether the S211A substitutionmight affect the subcellular localization of SOX9, we transfectedCOS-7 cells with a plasmid expressing either wild-type SOX9 orthe m1+2 mutant SOX9 with or without a PKA-C $alpha$ -expressing plasmidand examined the subcellular localization of SOX9 by immunofluorescence.Both wild-type SOX9 and m1+2 mutant SOX9 were nuclear (Fig. 5Aand B), findings that agree with those of an earlier study (20).Hence, the PKA phosphorylation site mutations did not affect thenuclear localization of SOX9. In addition, no change in the nuclearlocalization of the wild-type and m1+2 mutant SOX9s was seen incells cotransfected with PKA-C $alpha$ (Fig. 5C and D).

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FIG. 5. PKA phosphorylation of SOX9 does not affect its nuclear localization. COS-7 cells were transfected with expression plasmids for wild-type SOX9, m1+2 mutant SOX9, and PKA-C $alpha$ , as indicated. The top panels (A to D) show the nuclear localization of the wild-type and m1+2 mutant SOX9 proteins (yellow signal) visualized by immunofluorescence with SOX9 antibodies. The lower panels represent the same fields in which cell nuclei were stained with DAPI.

cAMP increases the activity of a Sox9-dependent chondrocyte-specific enhancer. To determine if PKA phosphorylation affects the activity of Sox9, we first tested whether cAMP signaling in RCS cells couldincrease the activity of a 48-bp Col2a1 enhancer that was previouslyshown to be dependent on Sox9 (20). Indeed, this 48-bp enhancer,which is chondrocyte specific in both DNA transfections and transgenicmice, binds Sox9 and becomes strongly active upon cotransfectionof SOX9 in nonchondrocytic cells; in addition, a mutant 48-bpenhancer, which has lost the ability to bind SOX9, is inactivein chondrocytes and is not activated by SOX9. In this experiment,we used the activity of a 48-bp Col2a1 enhancer construct to conducta functional assay of the transcriptional activity of SOX9. Treatmentof RCS cells with 1 mM 8-bromo-cAMP increased the activity ofthis Col2a1 chondrocyte-specific enhancer more than threefold(Fig. 6A). No increase in activity occurred in the presence of8-bromo-cAMP when only the 89-bp Col2a1 promoter, without the48-bp enhancer element, was used. Hence, the Sox9-dependent 48-bpCol2a1 enhancer seems to be a target for cAMP signaling in RCScells.

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FIG. 6. PKA and cAMP stimulate the activity of chondrocyte-specific Col2a1 enhancers. (A) 8-Bromo-cAMP increased the activity of the 48-bp Col2a1 enhancer in RCS cells. A luciferase reporter plasmid containing no (p89Luc) or four copies of a 48-bp chondrocyte-specific enhancer element (4x48-p89Luc) was transfected into RCS cells, and 4 h later, 1 mM 8-bromo-cAMP was added (+cAMP) or not ( $-$ ) to the culture medium for 8 h. Promoter activities were shown as the average plus standard deviation of triplicate transfections for A and B. (B) PKA-C $alpha$ increases the SOX9-dependent activation of the 48-bp Col2a1 enhancer in 10T1/2 fibroblasts. Expression plasmids for SOX9 and PKA-C $alpha$ were either transfected individually or cotransfected in a 1:4 ratio for a total of 16 h. Where indicated, the PKA inhibitor H8 was added to the medium for 12 h beginning 4 h after the start of transfection. (C) Cotransfected PKA-C $alpha$ increases the SOX9-dependent activation of the 100-bp Col2a1 enhancer in 10T1/2 fibroblasts. A luciferase reporter plasmid containing two copies of the 100-bp enhancer was cotransfected without ( $-$ ) or with the expression plasmids for SOX9 and PKA-C $alpha$ into 10T1/2 fibroblasts for a total of 16 h. Eight hours after the start of transfection, 1 mM 8-bromo-cAMP was added as indicated, and the mixture was incubated for an additional 8 h. Solid and hatched columns show the results of separate duplicate transfections.

PKA-C $alpha$ increases the activity of Sox9-dependent Col2a1 chondrocyte-specific enhancers. To further examine the molecular basis for the increase in activity of the 48-bp Col2a1 enhancer that is produced by cAMPin chondrocytes, we cotransfected the expression plasmids forSOX9 and PKA-C $alpha$ into 10T1/2 cells along with the 4x48-p89Luc Col2a1construct (Fig. 6B). In agreement with previous results (20),SOX9 stimulated the activity of the Col2a1 48-bp enhancer in thesecells, and cotransfection of PKA-C $alpha$ and SOX9 further increasedthis activity five- to sixfold. This increase was inhibited byH8, a PKA-specific inhibitor (18), in a dose-dependent manner(Fig. 6B). Moreover, cotransfection with PKA-C $alpha$ also increasedthe Sox9-dependent activities of two larger chondrocyte-specificCol2a1 enhancer constructs containing either two copies of a 100-bpsequence (Fig. 7C) or two copies of a 231-bp sequence (data notshown), each including the 48-bp element. Hence, the activitiesof the 48-bp and the larger Col2a1 Sox9-dependent enhancers werestimulated by PKA.

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FIG. 7. Mutations in the PKA phosphorylation sites of SOX9 decrease the ability of PKA to enhance SOX9 activation of the Col2a1 enhancer. COS-7 cells were transfected with the 4x48-p89Luc reporter construct and plasmids encoding wild-type SOX9 (lanes 3 and 7) or one of the SOX9 mutants (m1, lanes 4 and 8; m2, lanes 5 and 9; m1+2, lanes 6 and 10), and PKA-C $alpha$ (lanes 2 and 7 to 10). Lane 1 is a transfection with the 4x48-p89Luc reporter plasmid alone. Promoter activity was determined 12 h later and is shown as the average plus standard deviation of triplicate transfections. A Western blot of cell lysates was probed with SOX9 antibody to show the relative amounts of each of the SOX9 proteins. In cells cotransfected with PKA-C $alpha$ , the levels of SOX9 were 1.5 to 1.8 times higher than in cells not cotransfected with PKA-C $alpha$ . Promoter activities were normalized relative to the levels of SOX9 protein.

SOX9 mutations in each of the two PKA phosphorylation consensus sites inhibit the activation of SOX9 by PKA. To examine whether the increase in Sox9-dependent Col2a1 enhancer activity caused by PKA was directly due to phosphorylationof SOX9 by PKA, we tested the m1, m2, and m1+2 SOX9 mutants incotransfection experiments of COS-7 cells with the 4x48-p89Lucenhancer construct and a PKA-C $alpha$ expression plasmid. Western blottingindicated that similar levels of SOX9 were present in the lysatesof cells transfected with wild-type and mutant forms of SOX9,but in all cells cotransfected with PKA-C $alpha$ the levels of SOX9were approximately 1.5 to 1.8 times higher than in cells not cotransfectedwith PKA-C $alpha$ . It is possible that the vector expressing SOX9 containsa promoter element that is responsive to the forced expressionof PKA-C $alpha$ . We thus normalized the promoter activities relativeto the levels of SOX9 proteins. In cells not transfected withPKA-C $alpha$ , the levels of activation of the Col2a1 enhancer by wild-typeand mutant SOX9 were similar (Fig. 7). In contrast, mutationsin each PKA phosphorylation site of SOX9 inhibited the increasein Sox9-dependent Col2a1 enhancer activity produced by PKA. Theextent of this inhibition was more pronounced with the S211A mutation(m2 mutant), and the m1+2 mutant SOX9 had roughly equivalent activityto that without cotransfected PKA-C $alpha$ . In summary, these experimentsindicate that direct phosphorylation of SOX9 by PKA enhances SOX9'sability to transactivate Col2a1 chondrocyte-specific enhancers.Although the two PKA phosphorylation consensus sites in SOX9 areimportant, the S₂₁₁ site adjacent to the carboxyl-terminal endof the HMG DNA-binding domain seems to be more crucial in mediatingthe effects of PKA on transactivation of Col2a1 enhancers bySOX9.

Phosphorylation of SOX9 by PKA increases SOX9's DNA-binding activity to 18-bp and 48-bp Col2a1 enhancer elements. The DNA-binding activity of SRY, which contains an HMG DNA-binding domain with 50% identity to that of SOX9, was previouslyshown to be increased by PKA phosphorylation (6). We testedwhether DNA binding of SOX9 to either the 48-bp Col2a1 enhancerelement or an 18-bp subsegment of this enhancer (21), whichincludes the binding site for SOX9 (20), was increased afterPKA phosphorylation. Phosphorylation of SOX9 by PKA-C $alpha$ in vitroincreased its DNA binding to an 18-bp Col2a1 enhancer element(Fig. 8A). This increased binding was strongly inhibited by includingPKI in the phosphorylation reaction. In contrast, DNA bindingof the m1+2 mutant SOX9 was unchanged by incubation with PKA-C $alpha$ (Fig. 8B). The same result was obtained when a smaller segmentof recombinant SOX9 that included the HMG domain and the two PKAphosphorylation sites was used in DNA-binding experiments involvingboth the 48-bp and the 18-bp Col2a1 enhancer elements (data notshown). Thus, the PKA-dependent increase in DNA binding of SOX9may account for the observed PKA-dependent increase in transcriptionalactivation of SOX9-dependent Col2a1 enhancers.

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FIG. 8. Phosphorylation of SOX9 by PKA increases its efficiency of binding to the 18-bp Col2a1 enhancer element. Bacterially expressed and purified wild-type (wt) (A) or m1+2 mutant (B) SOX9 protein was incubated in vitro with PKA-C $alpha$ . Nonphosphorylated and phosphorylated proteins were then tested in an EMSA with the ³²P-labeled 18-bp Col2a1 enhancer element as a probe. A 100-fold excess of unlabeled 18-bp oligonucleotide competitor and PKI were added to the phosphorylation reactions, as indicated. The positions of wild-type and m1+2 mutant SOX9 complexes with the 18-bp probe are marked.

8-Bromo-cAMP mediates phosphorylation of Sox9 at serine 211 in rat chondrosarcoma cells. The specificity of a phosphospecific antibody for a SOX9 peptide in which S₂₁₁ was phosphorylated is illustrated in Fig. 9A.In extracts of COS-7 cells transfected with a wild-type SOX9 expressionplasmid, the phosphospecific antibody showed a very weak signal.The intensity of this signal increased markedly when extractsof COS-7 cells that had been cotransfected with SOX9 and PKA-C $alpha$ expression plasmids were tested. No signal was seen in extractsof cells cotransfected with the m2 SOX9 mutant carrying the S211Amutation and PKA-C $alpha$ , demonstrating the complete specificity ofthe antibody. Extracts of cells transfected with the m1 SOX9 mutantand PKA-C $alpha$ showed the same signal intensity as extracts of cellstransfected with wild-type SOX9, whereas those of cells transfectedwith the m1+2 mutant and PKA-C $alpha$ showed no signal. In addition,the SOX9 phosphospecific antibody did not recognize SOX9 madein E. coli. Thus, the antibody specifically reacted with SOX9that was phosphorylated at S₂₁₁. Our experiments demonstrate thatcotransfection with PKA-C $alpha$ led to phosphorylation of SOX9 at S₂₁₁.Moreover, adding 8-bromo-cAMP to RCS cells produced a marked increasein signal intensity (Fig. 9B), directly demonstrating that signalingby cAMP results in phosphorylation at S₂₁₁ of endogenous Sox9.

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FIG. 9. Phosphorylation of Sox9 at S₂₁₁ in intact cells. (A) Recombinant SOX9 protein made in E. coli and extracts from COS-7 cells that were transfected with plasmids expressing wild-type (wt) SOX9 or mutant SOX9 proteins and a plasmid expressing PKA-C $alpha$ , as indicated, were resolved by SDS-10% PAGE followed by Western blotting with SOX9.P antibody (Ab) at a dilution of 1:1,000. The antibodies were stripped off the blots, and the membranes were reprobed with another SOX9 antibody as described previously (20). In A and B, the 68-kDa mobility of Sox9 is indicated by an arrow. (B) Cell extracts from RCS cells, untreated or treated with two different concentrations of 8-bromo-cAMP for 8 h, were used for Western blotting.

Sox9 phosphorylated at S₂₁₁ is present in the prehypertrophic zone of the growth plate. In order to determine whether Sox9 was phosphorylated at S₂₁₁ in the growth plate in vivo during chondrocyte differentiation,we used the SOX9 phosphospecific antibody to perform an immunohistochemicalanalysis of the growth plate of 16.5 dpc mouse embryo hind legs.Immunohistochemistry with the SOX9 antibody directed against anepitode located at the carboxyl terminus of SOX9 (22) showedthat Sox9 was evenly distributed in the cells along the growthplate, including the resting, proliferative, and prehypertrophiczones, but was absent in the hypertrophic zone (Fig. 10A). Theseresults are in perfect agreement with those of previous RNA insitu hybridizations (27, 37). In contrast, Sox9 phosphorylatedat S₂₁₁ localized mainly in the prehypertrophic zone (Fig. 10B).

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FIG. 10. Sox9 is phosphorylated at S₂₁₁ in the prehypertrophic zone of the growth plate in vivo. (A) Immunohistochemistry of a hind limb section of E 16.5 mouse embryo with SOX9 antibodies. Sox9 is evenly distributed in the cells of the resting, proliferative (P), and prehypertrophic (Pre-hy) zones of the growth plate. No Sox9 protein was observed in the hypertrophic (hy) zone. (B) Immunohistochemistry of a parallel section with SOX9.P antibodies. Sox9 phosphorylated at S₂₁₁ was present in the prehypertrophic zone of the growth plate. Bars, 50 µm.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The results of our yeast two-hybrid screen indicating interactions between SOX9 and PKA-C $alpha$ prompted us to hypothesize thatSOX9 might be a target for PKA phosphorylation. Several linesof evidence show that cAMP is an important signaling moleculein chondrocyte differentiation. For example, PTHrP, which inhibitsthe transition from prehypertrophic chondrocytes to hypertrophicchondrocytes (12, 16), signals by increasing the intracellularconcentration of cAMP, since the PTH/PTHrP receptor is a G protein-coupledreceptor that activates the adenylate cyclase enzyme (11). Inaddition, in cell culture cAMP increases the expression of severalchondrocyte marker genes, including Col2a1, that are targets ofSox9 in chondrocytes (3, 14). Since PKA has also been shownto modulate signaling by sonic hedgehog (7, 9), one canpostulate that, by analogy, cAMP might also be important in signalingby indian hedgehog (Ihh), which has a key role in controllingthe expression of PTHrP (16). Moreover, signaling by bone morphogeneticproteins, which have the ability to induce the whole cascade ofchondrocyte differentiation in vivo and in vitro, activates PKAin cultured chondrocytes (18). Because Sox9 has an essentialrole in chondrocyte differentiation, its phosphorylation by PKAmight provide a mechanism to control its activity. We thereforeinvestigated the potential role of PKA phosphorylation in modulatingSox9activity.

SOX9 contains two consensus PKA phosphorylation sites that are conserved in humans, mice, and chickens. We showed that eachsite can be phosphorylated by PKA-C $alpha$ in vitro, because each ofthe single SOX9 mutants m1 and m2 could be phosphorylated by PKA-C $alpha$ ,whereas the double mutant m1+2 could not. We next determined thatSOX9 is also phosphorylated by PKA in intact cells. Indeed, cotransfectionof wild-type SOX9 with PKA-C $alpha$ produced an increase in SOX9 phosphorylationthat was not observed with the m1+2 mutant SOX9. Our finding thatthe m1+2 mutant SOX9 was phosphorylated suggests that SOX9 canbe phosphorylated at other sites in intact cells, presumably bykinases other than PKA. Consensus phosphorylation sites for PKC,PKG, and casein kinase II are present in the SOX9 sequence, asdetermined by computer analysis (data not shown). Evidence thatSOX9 is phosphorylated at S₂₁₁ in intact cells was obtained byusing a phosphospecific antibody. This site became highly phosphorylatedin cells cotransfected with SOX9 and PKA-C $alpha$ but not in cells transfectedwith SOX9 only. Moreover, the addition of 8-bromo-cAMP to RCScells induced a marked increase in the phosphorylation of endogenousSox9 at S₂₁₁.

Since S₂₁₁ is part of a Sox9 nuclear localization signal (32), the phosphorylation status of Sox9 may be important for nucleartranslocation. Our immunofluorescence experiments demonstratedthat the nuclear localization of the m1+2 SOX9 mutant was identicalto that of wild-type SOX9 in transfected COS-7 cells. Moreover,the nuclear localization of SOX9 was not different in cells thatwere cotransfected with PKA-C $alpha$ . We therefore concluded that PKAphosphorylation has no effect on the nuclear localization ofSOX9.

We used the activity of Sox9-dependent Col2a1 enhancer elements in DNA transfection experiments as a functional assay to testwhether cAMP signaling increased the transcriptional activityof Sox9. We found that treating RCS cells with 8-bromo-cAMP increasedthe activity of a construct carrying four copies of the 48-bpCol2a1 enhancer; similarly, cotransfection of SOX9 with PKA-C $alpha$ in COS-7 cells and other fibroblasts also stimulated severalfoldthe Sox9-dependent activity of this and two larger Col2a1 enhancerelements. Moreover, adding a PKA inhibitor to these cotransfectionexperiments strongly inhibited this stimulation. Cotransfectionof mutant forms of SOX9 together with PKA-C $alpha$ resulted in a lesserdegree of stimulation than that produced by PKA and wild-typeSOX9. Although both mutation 1 (S₆₄) and mutation 2 (S₂₁₁) decreasedthe PKA-enhanced activity, mutation 2 did so to a greater extent,suggesting that S₂₁₁ has a greater role than S₆₄ in mediatingthe effect of PKA phosphorylation. With SOX9 containing both mutations,there was practically no stimulation by PKA. The presence of thesemutations did not affect SOX9 activity in the absence of PKA,since wild-type SOX9 and the three different SOX9 mutants activatedthe Col2a1 48-bp enhancer to similarlevels.

Together, these experiments strongly suggest that phosphorylation of SOX9 by PKA increases the transcriptional activity ofSOX9. This increase in SOX9 transcriptional activity is unlikelyto be due to stabilization of SOX9, because similar levels ofSOX9 were found in cells expressing wild-type and mutant SOX9proteins. The increased transcriptional activity of SOX9 couldbe accounted for by the increased efficiency of DNA binding ofSOX9 that was observed upon PKA-C $alpha$ phosphorylation. It is alsopossible that phosphorylated SOX9 interacts more efficiently withcomponents of the transcriptional machinery. In addition, activePKA also results in phosphorylation of several other transcriptionfactors (4), some of which may interact more efficiently withphosphorylated SOX9 and increase the observed activity of Sox9-dependentCol2a1enhancers.

The PTH/PTHrP receptor is expressed in a relatively narrow band in the prehypertrophic zone of growth plate cartilages. Insitu hybridization experiments have shown that the levels of Col2a1mRNA are higher in this zone than in other areas of the growthplate (17). Since cAMP signaling is one the major signalingpathways of the PTH/PTHrP receptor, we speculate that PKA phosphorylationof Sox9 may increase the transcriptional activity of Sox9 in thiszone, which would result in higher levels of Col2a1 mRNA. Ourimmunohistochemical analysis using the SOX9 phosphospecific antibodyshowed a strong signal for Sox9 phosphorylated at S₂₁₁ in theprehypertrophic zone of the growth plate where the PTH/PTHrP receptoris expressed (17). In a control experiment, an antibody againstthe carboxyl terminus of SOX9 showed that Sox9 was evenly distributedthroughout the resting, proliferative, and prehypertrophic zones.Our results therefore strongly suggest that PTHrP might be a physiologicalsignal for the PKA-mediated phosphorylation of Sox9 in the growthplate. Since the major function of PTHrP is to inhibit furtherdifferentiation of chondrocytes into hypertrophic chondrocytes,we speculate that the increase in activity of the master chondrogenicfactor Sox9 by PKA phosphorylation could mediate at least someof the effects of PTHrP in the growth plate by maintaining thecells as nonhypertrophicchondrocytes.

	ACKNOWLEDGMENTS

This work was funded by NIH grants R01 AR42909 and P01 AR 42919-02 to Benoit de Crombrugghe. Véronique Lefebvre was supportedby the Arthritis Foundation. DNA sequencing was performed by theUniversity of Texas M. D. Anderson Cancer Center core sequencingfacility, which is supported by NCI grant CA16672.

We thank James H. Kimura for the RCS cells, Ami Aronheim for the SRS plasmids and the cdc25-2 yeast strain, and Michael Uhlerfor the PKA-C $alpha$ cDNA plasmid. We are grateful to Sankar N. Maityand Kazuhisa Nakashima for valuable advice throughout the workand to Shane Zhao for help in computer analysis of SOX9 proteinsequences. We also thank Heidi Eberspaecher and Gerald Pinerofor their help in the immunohistochemistry and Patricia Arubalezefor help in typing themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Genetics, The University of Texas M. D. Anderson Cancer Center,1515 Holcombe Boulevard, Box 11, Houston, TX 77030. Phone: (713)792-2590. Fax: (713) 794-4295. E-mail: bdecromb{at}mdanderson.org.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Passeron, T., Valencia, J. C., Bertolotto, C., Hoashi, T., Le Pape, E., Takahashi, K., Ballotti, R., Hearing, V. J. (2007). SOX9 is a key player in ultraviolet B-induced melanocyte differentiation and pigmentation. Proc. Natl. Acad. Sci. USA 104: 13984-13989 [Abstract] [Full Text]
Hirao, M., Tamai, N., Tsumaki, N., Yoshikawa, H., Myoui, A. (2006). Oxygen Tension Regulates Chondrocyte Differentiation and Function during Endochondral Ossification. J. Biol. Chem. 281: 31079-31092 [Abstract] [Full Text]
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Chikuda, H., Kugimiya, F., Hoshi, K., Ikeda, T., Ogasawara, T., Shimoaka, T., Kawano, H., Kamekura, S., Tsuchida, A., Yokoi, N., Nakamura, K., Komeda, K., Chung, U.-i., Kawaguchi, H. (2004). Cyclic GMP-dependent protein kinase II is a molecular switch from proliferation to hypertrophic differentiation of chondrocytes. Genes Dev. 18: 2418-2429 [Abstract] [Full Text]
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Huang, W., Lu, N., Eberspaecher, H., de Crombrugghe, B. (2002). A New Long Form of c-Maf Cooperates with Sox9 to Activate the Type II Collagen Gene. J. Biol. Chem. 277: 50668-50675 [Abstract] [Full Text]
Rehberg, S., Lischka, P., Glaser, G., Stamminger, T., Wegner, M., Rosorius, O. (2002). Sox10 Is an Active Nucleocytoplasmic Shuttle Protein, and Shuttling Is Crucial for Sox10-Mediated Transactivation. Mol. Cell. Biol. 22: 5826-5834 [Abstract] [Full Text]
Davies, S. R., Sakano, S., Zhu, Y., Sandell, L. J. (2002). Distribution of the Transcription Factors Sox9, AP-2, and [Delta]EF1 in Adult Murine Articular and Meniscal Cartilage and Growth Plate. J. Histochem. Cytochem. 50: 1059-1065 [Abstract] [Full Text]
Weston, A. D., Chandraratna, R. A.S., Torchia, J., Underhill, T. M. (2002). Requirement for RAR-mediated gene repression in skeletal progenitor differentiation. JCB 158: 39-51 [Abstract] [Full Text]
Ray, B. K., Chen, J., Ray, A. (2001). Catalytic Subunit of Protein Kinase A Is an Interacting Partner of the Inflammation-Responsive Transcription Factor Serum Amyloid A-Activating Factor-1. J. Immunol. 167: 2343-2348 [Abstract] [Full Text]
Panda, D. K., Miao, D., Lefebvre, V., Hendy, G. N., Goltzman, D. (2001). The Transcription Factor SOX9 Regulates Cell Cycle and Differentiation Genes in Chondrocytic CFK2 Cells. J. Biol. Chem. 276: 41229-41236 [Abstract] [Full Text]
Huang, W., Chung, U.-i., Kronenberg, H. M., de Crombrugghe, B. (2001). The chondrogenic transcription factor Sox9 is a target of signaling by the parathyroid hormone-related peptide in the growth plate of endochondral bones. Proc. Natl. Acad. Sci. USA 98: 160-165 [Abstract] [Full Text]

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