Sox10, a Novel Transcriptional Modulator in Glial Cells

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The Journal of Neuroscience, January 1, 1998, 18(1):237-250

Sox10, a Novel Transcriptional Modulator in Glial Cells
Kirsten Kuhlbrodt, Beate Herbarth, Elisabeth Sock, Irm Hermans-Borgmeyer, and Michael Wegner
Zentrum für Molekulare Neurobiologie, Universität Hamburg, D-20246 Hamburg, Germany

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Sox proteins are characterized by possession of a DNA-binding domain with similarity to the high-mobility group domain ofthe sex determining factor SRY. Here, we report on Sox10, a novelprotein with predominant expression in glial cells of the nervoussystem. During development Sox10 first appeared in the formingneural crest and continued to be expressed as these cells contributedto the forming PNS and finally differentiated into Schwann cells.In the CNS, Sox10 transcripts were originally confined to glialprecursors and later detected in oligodendrocytes of the adultbrain. Functional studies failed to reveal autonomous transcriptionalactivity for Sox10. Instead, Sox10 functioned synergisticallywith the POU domain protein Tst-1/Oct6/SCIP with which it is coexpressedduring certain stages of Schwann cell development. Synergy dependedon binding to adjacent sites in target promoters, was mediatedby the N-terminal regions of both proteins, and could not be observedbetween Sox10 and several other POU domain proteins. Interestingly,Sox10 also modulated the function of Pax3 and Krox-20, two othertranscription factors involved in Schwann cell development. Wepropose a role for Sox10 in conferring cell specificity to thefunction of other transcription factors in developing and matureglia.

Key words: POU; Sox; synergy; neural crest; Schwann cell; oligodendrocyte

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Glial cells and their development have been studied extensively both in the CNS and in the PNS (for review, see Pfeiffer etal., 1993; Mirsky and Jessen, 1996; Zorick and Lemke, 1996). Inthe PNS, migrating neural crest cells join axons that grow outfrom the ventral part of the neural tube early during developmentand proliferate along these tracts (LeDouarin, 1982). By mouseembryonic day 12-13 (E12-E13), these neural crest-derived cellsalready loosely contact several axon bundles and have turned intoSchwann cell precursors (Jessen et al., 1994). By E15-E16 mostof these cells have progressed to the embryonic Schwann cell stageand have started to segregate and subdivide axon bundles. A fractionof Schwann cells remains in contact with multiple axons and givesrise to nonmyelinating Schwann cells, which in the adult surroundseveral slow conducting small-caliber axons with simple extensionsof their plasma membrane. Those in contact with large-caliberaxons achieve a 1:1 relationship around birth. Shortly thereafter,this latter group ceases to proliferate and differentiates intomyelinating Schwann cells, characterized by the expression ofmyelin genes and the elaboration of a multilayered myelin sheath(Lemke, 1988).

Several transcription factors have been shown to be involved in the development of Schwann cells, including the paired domainprotein Pax3 (Kioussi et al., 1995), the zinc finger protein Krox-20(Topilko et al., 1994), and the POU domain protein Tst-1/Oct6/SCIP(Monuki et al., 1989; Bermingham et al., 1996; Jaegle et al.,1996). From comparison of expression patterns and mouse mutantphenotypes it was concluded that these transcription factors functionat distinct stages of Schwann cell development, with Tst-1/Oct6/SCIPbeing active after Pax3 but before Krox-20 (Blanchard et al.,1996; Zorick et al., 1996).

The fact that Tst-1/Oct6/SCIP is much more active in glia than in several other cell types has been taken as evidence forthe existence of accessory proteins in glia that modulate theactivity of Tst-1/Oct6/SCIP in a cell type-specific manner (Monukiet al., 1993; Sock et al., 1996b). Recent analysis in embryonalstem cells suggested that Sox proteins might function as celltype-specific accessory proteins for POU domain proteins (Yuanet al., 1995). These proteins, which contain as their DNA-bindingdomain a divergent form of high-mobility group (HMG) domain firstidentified in the sex determining factor SRY (Gubbay et al., 1990)often exhibit a highly restricted tissue distribution (Pevny andLovell-Badge, 1997) and frequently function in concert with othertranscription factors (Kamachi et al., 1995; Yuan et al., 1995).To identify cell type-specific accessory proteins for Tst-1/Oct6/SCIP,we decided to look at Sox proteins in Schwann cells.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Cell culture. Oligodendroglial cultures were prepared from the brains of 1-d-old Wistar rats as described (McCarthy and DeVellis,1980) with minor modifications (Sock et al., 1997). Schwann cellswere isolated from 3-d-old rats by the method of Brockes et al.(1979) as modified by Porter et al. (1986). Rat CG-4 cells (Louiset al., 1992) were grown on poly-L-ornithine-coated plates inDMEM containing N1 supplement (5 µg/ml transferrin, 16 µg/ml putrescine,60 ng/ml progesterone, 50 ng/ml selenium, and 5 µg/ml insulin),10 ng/ml PDGF, and 5 ng/ml basic FGF (bFGF) (Louis et al., 1992).Differentiation of CG-4 cells was induced by omitting PDGF andbFGF from the medium. U138 human glioblastoma cells were propagatedin RPMI-1640 medium supplemented with 10% FCS. All other celllines including P19 embryonal carcinoma, NB4 1A3, N1E-115, Neuro2Aneuroblastomas, C6, HJC gliomas, 33B oligodendroglioma, 3T3, Rat1fibroblasts, B103, and COS7 cells were maintained in DMEM supplementedwith 10% FCS.

RNA preparation, reverse transcription PCR, and library screening. RNA was isolated from cell cultures and dissected mouseand rat tissues using Trizol reagent (Life Technologies, Gaithersburg,MD).

For the identification of Sox genes in glial cells, 2 µg of total RNA from primary Schwann cells was reverse-transcribed for1 hr at 42°C using 400 U Moloney murine leukemia virus reversetranscriptase, 45 pmol of oligo-dT primer, and 0.5 mM dNTP in30 µl of (in mM): 50 Tris-HCl, pH 8.3, 75 KCl, 3 MgCl₂, and 1DTT. Two microliters of this reaction were amplified using thedegenerate primers 5 $'$ -AAGGCCGGATCCATGAA(CT)GC(ACT)TT(CT)AT(AGT)GT(TGCA)TGG-3 $'$ and 5 $'$ -AAGGCCGGATCC(TGCA)GGTCTT(AG)TA(CT)TT(AG)TA(AG)TC(TGCA)GG-3 $'$ (Yuan et al., 1995). In addition to 40 pmol of each degenerateprimer, PCRs contained 0.2 mM dNTP and 1 U of Taq DNA polymerasein 50 µl of (in mM): 10 Tris-HCl, pH 8.3, 50 KCl, and 2 MgCl₂.After an initial denaturation step for 1 min at 94°C, 25 cycleswere performed with each cycle consisting of a denaturation (1min at 94°C), an annealing step (1 min at 45°C), and an elongationstep (1 min at 72°C). Amplification products were subcloned intothe BamHI site of pBluescript KS+ (Stratagene, La Jolla, CA) andsequenced. The 200 bp fragment corresponding to the HMG domainof Sox10 was radiolabeled and used to screen an oligo-dT-primedcDNA library constructed from poly(A⁺) RNA of undifferentiated CG-4 cells in $lambda$ -Ziplox (Life Technologies).Plasmids were excised from five independent positive $lambda$ phagesaccording to the manufacturer's instructions. All were found tocontain the Sox10 HMG domain. The longest insert had a size of3030 bp and covered all regions present in other inserts. Itssequence was determined in full and deposited in EMBL/GenBankunder accession number AJ001029.

Plasmids. Plasmid pZL1/Sox10 was derived from screening the CG-4 cDNA library, and contained the 3030 bp Sox10 cDNA. The samefragment was inserted into the EcoRI site of pCMV5, yielding themammalian expression plasmid pCMV/Sox10. Plasmid pCMV/Sox10 $Delta$ Nwas created by placing eukaryotic translation initiation consensusand T7 tag (Novagen, Madison, WI) immediately in front of methionine90 in the context of pCMV5. In the case of pCMV/Sox10HMG, translationinitiation consensus and T7 tag were added onto the first residueof the HMG domain of Sox10, and a stop codon was introduced immediatelybehind the HMG domain. The HMG domain of Sox10 was also insertedinto pGEX-KG after PCR-directed introduction of flanking BamHIand XhoI sites. Bacterial expression of Sox10 holoprotein requiredthe cloning of Sox10 coding sequences between EcoRI and XhoI sitesof pET28 (Novagen).

Eukaryotic expression plasmids pCMV/Brn-3.0, pCMV/Tst-1, and its mutants pCMV/Tst-1 $Delta$ N, pCMV/Tst-1 $Delta$ P_S, and pCMV/Tst-1 $Delta$ C havebeen described (Gerrero et al., 1993; Sock et al., 1996a). pCMV/Brn-1contained the open reading frame of rat Brn-1 as part of a 2.2kb EcoRI-NsiI fragment. pCMV/Oct-3/4 was generated by insertingthe cDNA for Oct-3/4 (a gift from P. Matthias, Friedrich MiescherInstitut, Basel, Switzerland) as an EcoRI-XhoI fragment into pCMV5.pCMV/Sox4 contained the open reading frame of rat Sox4 as a 2.0kb EcoRI fragment. Plasmid pCMV/Sox2 was a gift of R. Lovell-Badge(MRC, London, UK). Fragments corresponding to the open readingframe of Krox-20 and Pax3 were amplified by PCR from rat Schwanncell cDNA and inserted between HindIII and BamHI sites (pCMV/Krox-20)or in the EcoRI site (pCMV/Pax3) of pCMV5.

pCMVGal4 contained coding sequences for the DNA-binding domain of the yeast Gal4 protein (Schreiber et al., 1997). Insertionof Sox10 and Tst-1/Oct6/SCIP sequences led to an in-frame fusionof both open reading frames, with Sox10 or Tst-1/Oct6/SCIP afterGal4 sequences. Fragments corresponding to full-length Sox10,its N-terminal region (amino acids 1-101), and its C-terminalregion (amino acids 181-466) were generated by PCR with flankingEcoRI and KpnI sites and inserted into pCMVGal4, yielding pCMVGal4/Sox10,pCMVGal4/Sox10 N, and pCMVGal4/Sox10 C, respectively. The N-terminalpart of Tst-1/Oct6/SCIP (amino acids 1-240) was cloned betweenBamHI and NheI sites of pCMVGal4 after the introduction of correspondingrestriction sites into the Tst-1/Oct6/SCIP sequence by site-directedmutagenesis.

The Gal4-responsive luciferase reporter (3xUAS luc) contained three tandem copies of a Gal4 binding site in front of the ratprolactin minimal promoter (Schreiber et al., 1997). Other luciferasereporters used in this study were constructed by inserting oligonucleotidescorresponding to SX, herpes simplex virus octamer (HSVoct), FXO,FXP, or FXK (for sequences, see Figs. 6, 7, 8, 10) into pTATAluc,which carried the luciferase gene under the control of the $beta$ -globinminimal promoter (Schreiber et al., 1997). The resulting luciferaseplasmids contained two copies (2xFXK luc) or three copies (3xSXluc, 3xHSVoct luc, 3xFXO luc, and 3xFXP luc) of each individualsite.

Northern blot analysis. For RNA blot analysis, 10 µg of total RNA was separated on formaldehyde-containing 1% agarose gels,blotted onto Duralose UV membranes (Stratagene), and hybridizedto ³²P random-labeled probes according to standard procedures. Thefollowing probes were used: a 1.45 kb EcoRI fragment from pMBP1(Roach et al., 1983), a 0.7 kb PstI-XbaI fragment from pBKS/GAPDH(Sock et al., 1997), a 3.0 kb EcoRI fragment corresponding tothe complete sequence of Sox10, and a 1.75 kb NcoI-EcoRI fragmentcorresponding to the second half of the Sox10 cDNA devoid of theHMG domain.

In situ hybridization histochemistry. Embryos (E6.5-E18.5) and neonates [postnatal days 0-21 (P0-P21)] from natural matingsbetween inbred CD-1 mice (Charles River Laboratories, Wilmington,MA) were used. The midday of the occurrence of a vaginal plugwas defined as E0.5 and the day of birth as P0. For in situ hybridizationon sections, the animals were frozen on dry ice, and 10 µm sectionswere prepared on a cryostat (Leitz, Wetzlar, Germany). Adult mouseand rat brains were sectioned at 15 µm. In situ hybridizationusing ³⁵S-uridine triphosphate (UTP)-labeled riboprobes was performedas described (Süsens et al., 1997). Sections were exposed toBioMax MR film for 3 d. For higher-resolution studies, the sameslides were dipped in Kodak (Rochester, NY) NTB-2 nuclear emulsion,developed in Dektol developer (Kodak) after 2-3 weeks of exposure,and subsequently stained with Giemsa (Sigma, St. Louis, MO). Forcomparison of neuronal and glial expression patterns, adjacent10 µm sections were hybridized with probes for Sox10 and the neuronalmarker SorLA (Hermans-Borgmeyer et al., 1997; Mörwald et al.,1997). Dark-field images of these sections were scanned, assignedfalse colors, and superimposed on the corresponding bright-fieldimage using Adobe Photoshop software for Macintosh computers.

Whole-mount in situ hybridizations using digoxygenin (DIG)-UTP-labeled probes were performed on embryos as described (Wilkinson,1992; Rosen and Beddington, 1993) with modifications (Parr etal., 1993). Up to E10.5 proteinase K treatment was omitted. The1.75 kb antisense riboprobe was transcribed by SP6 polymeraseafter linearizing pZL1/Sox10 with NcoI and corresponded to thesecond half of the Sox10 cDNA without the HMG domain. For thesense probe, pZL1/Sox10 was transcribed by T7 polymerase afterBamHI linearization. Transcription reactions were performed usingthe Ambion transcription kit for the production of radioactiveprobes and the Boehringer Mannheim (Mannheim, Germany) DIG labelingkit for the production of DIG-labeled probes. Morphological structureswere identified by reference to Rugh (1990) and Kaufman (1992).

Transfections and luciferase assays. U138 cells were transfected by the calcium phosphate technique as described (Renner etal., 1994). COS cells were transfected by the DEAE-dextran techniqueusing a concentration of 500 µg/ml DEAE-dextran followed by chloroquinetreatment (Sock et al., 1996b). For luciferase assays, cells weretransfected with 2 µg of luciferase reporter plasmid and 0.05-2µg of cytomegalovirus (CMV) expression plasmid per 60 mm plate.The total amount of plasmid was kept constant using empty CMVvector. Cells were harvested 48 hr after transfection, and extractswere assayed for luciferase activity (Renner et al., 1994).

Preparation of recombinant proteins and antisera. Full-length Sox10 protein was produced in Escherichia coli BL21 DE3 as ahexahistidine fusion protein using the pET expression system (Novagen).Purified, denatured Sox10 holoprotein was used as antigen to raisean antiserum in rabbit. Expression of a fusion protein betweenglutathione S-transferase (GST) and the HMG domain of Sox10 frompGEX/Sox10 in E. coli DH5 $alpha$ and purification procedures were asdescribed (Renner et al., 1994).

Protein extracts and Western blots. Nuclear and whole-cell extracts were prepared as described (Sock et al., 1997). Fifteenmicroliters of nuclear or whole-cell extract (~4 mg/ml) were size-fractionatedon SDS-12% polyacrylamide gels and used for Western blot analysis(Sock et al., 1996a). The rabbit antiserum against Sox10 or amouse monoclonal antibody against the DNA-binding domain of Gal4(Clontech, Palo Alto, CA) served as primary antibodies, each ata dilution of 1:3000. The enhanced chemiluminescence system (Amersham,Arlington Heights, IL) was used for detection.

Electrophoretic mobility shift assay. The SX, HSV oct, and FXO oligonucleotides (for sequences, see Figs. 6, 7, 8) were usedas probes. In general, 0.5 ng of ³²P-labeled probe was incubated with 10 ng of GST fusion proteinor 400 ng of nuclear extract from transfected COS cells for 20min on ice in a 20 µl reaction mixture containing 10 mM HEPES,pH 8.0, 5% glycerol, 50 mM NaCl, 5 mM MgCl₂, 2 mM DTT, 0.1 mMEDTA, 4 µg of bovine serum albumin, and 2 µg of poly(dGdC) asunspecific competitor. In some cases, antiserum (0.5 µl) was addedto the reaction, and incubation was continued for an additional5 min before loading onto native 4% polyacrylamide gels. Electrophoresiswas performed in 0.5 × Tris-borate-EDTA (in mM: 45 Tris, 45 boricacid, and 1 EDTA, pH 8.3) at 180 V for 1.5 hr. Gels were driedand exposed for autoradiography.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Identification of Sox10

To identify Sox proteins present in PNS glia, we exploited the fact that all Sox proteins contain a highly conserved SRY-relatedHMG domain (Pevny and Lovell-Badge, 1997). Using cDNA preparedfrom primary Schwann cell cultures, we amplified sequences correspondingto the HMG domain of Sox proteins in PCRs using a pair of previouslydescribed degenerate primers (Yuan et al., 1995). Sequencing ofPCR products (Fig. 1A) revealed that more than two-thirds correspondedto the HMG domain of Sox10 (Wright et al., 1993). No other Soxprotein was detected in comparable amounts, although the degenerateprimers matched Sox10 sequences and other Sox sequences equallywell.

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Figure 1. Identification of Sox10. A, Sequence analysis of clones obtained from Schwann cell cDNA by PCR with Sox-specific degenerateprimers. B, Structure of the Sox10 cDNA (EMBL/GenBank accessionnumber AJ001029) and amino acid sequence deduced from the openreading frame between positions 583 and 1980. C, Comparison ofthe amino acid sequence of Sox10 with those of the related mouseSox9 (Wright et al., 1995), mouse Sox8 (Wright et al., 1993),and rainbow trout SoxP1 (Ito et al., 1995). Exact matches betweenSox10 and the aligned sequences are marked by asterisks. The aminoacids corresponding to the HMG domain are boxed. D, Detectionof endogenous Sox10 in nuclear extracts of 33B rat oligodendrogliomaand B103 tumor cells by Western blot using a rabbit antiserumraised against Sox10 holoprotein. A nuclear extract from COS cellstransfected with a Sox10 expression plasmid served as a positivecontrol. Numbers on the left indicate sizes of molecular weightmarkers in kilodaltons.

Because the isolation of Sox10 cDNA sequences other than those within the HMG domain had not been reported, we used the PCRproduct to screen a rat CG-4 cDNA library. The largest of thepositive isolates had a size of 3030 bp. We detected a singleopen reading frame of 466 amino acids starting at bp 583 and extendingto bp 1980 (Fig. 1B). An in-frame stop codon was present in frontof the open reading frame at bp 190. The encoded protein containedan HMG domain in the N-terminal half that was identical to thepublished sequence of the Sox10 HMG domain (Wright et al., 1993).Sox10 belongs to the same subgroup of Sox proteins as Sox8 andSox9, as indicated by the fact that the HMG domains of all threeproteins share >90% identity (Wright et al., 1993). Sequence similaritieswere apparent even outside the HMG domain (Fig. 1C). When aminoacid sequences of rat Sox10 and mouse Sox9 (Wright et al., 1995)were aligned with sequences of SoxP1, the putative Sox8 orthologfrom rainbow trout (Ito et al., 1995), we detected three additionalregions with significant sequence conservation. One of them correspondedto amino acids 233-306 of Sox10 with 61% identity over a stretchof 74 amino acids, and a second one corresponded to the C-terminalregion of Sox10 with 41% identity over a stretch of 66 amino acids.This latter region corresponded to the transactivation domainof Sox9 (Südbeck et al., 1996). Most conspicuously, all threeproteins were 78% identical over a region of 36 amino acids thatdirectly preceded the HMG domain. This region might constitutea class-specific extension of the HMG domain in this particularsubgroup of Sox proteins.

The open reading frame of 466 amino acids predicted a molecular weight of ~50 kDa for Sox10. To be able to detect Sox10 proteinin cells, we generated a rabbit antiserum against Sox10 holoprotein.This antiserum recognized a protein of ~56 kDa in nuclear extractsfrom several cell lines, including B103 and 33B. A protein ofidentical size was detected in extracts from COS cells transfectedwith the complete Sox10 cDNA under the control of a CMV promoter,not however, in mock-transfected COS cells (Fig. 1D; data notshown). Thus, Sox10 has a slightly lower electrophoretic mobilitythan predicted from its amino acid sequence.

Tissue distribution of Sox10

To assess Sox10 expression in rodents, we prepared total cellular RNA from several mouse and rat tissues and analyzed theseRNAs by Northern blot for the presence of Sox10 message. The resultof this survey indicated that expression of the 3 kb Sox10 mRNAis largely restricted to the nervous system (Fig. 2A). Sox10 transcriptswere abundant in brain but not detectably expressed in heart,skeletal muscle, testis, liver, or the adrenal gland (Fig. 2A)or in spleen, lung, or kidney (data not shown). Integrity andequal loading of the RNAs were confirmed by rehybridization witha glyceraldehyde phosphate dehydrogenase (GAPDH) probe. Closerexamination of dissected brain regions indicated that Sox10 messagewas expressed throughout the whole brain (Fig. 2B). However, variationsin expression levels were seen between various parts of the brain.In general, abundance of Sox10 mRNA correlated with the relativecontent of myelinated fiber tracts in the respective region, beingfor instance high in pons or olfactory bulb and relatively lowin cortex and cerebellum.

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Figure 2. Tissue distribution of Sox10 mRNA. Total cellular RNA from the indicated rat tissues (A) or regions of adult rat brain (B)was analyzed for the expression of Sox10 mRNA by Northern blot.Filters were hybridized consecutively with probes specific forSox10 (top panel) and GAPDH (bottom panel). The region designatedmidbrain in B contained thalamus, hypothalamus, superior and inferiorcolliculi, as well as surrounding regions. Hippocampus includedfimbria and part of the corpus callosum. Negative tissues notshown in A included spleen, lung, and kidney. Identical resultswere obtained with mouse tissues.

To define cell types in which Sox10 is predominantly expressed, we performed a second survey with total RNAs from a varietyof neural and non-neural cells or cell lines (Fig. 3). BecauseSox10 was originally detected by PCR in cDNA prepared from Schwanncells, we first analyzed whether Sox10 message was present inRNA from cultured Schwann cells (Fig. 3A). An abundant 3 kb transcriptwas indeed detected in these cells. No Sox10 mRNA was found in3T3 or Rat1 fibroblasts. Similarly, the embryonal carcinoma cellline P19 and the neuroblastomas NB4 1A3, N1E-115, and Neuro2Ascored as negative. This apparent absence in neuroblastomas contrastedsharply with the strong hybridization signal obtained for 33Boligodendroglioma and for C6 and HJC glioma cell lines derivedfrom either rat or hamster. We also observed Sox10 expressionin the tumor cell line B103. Although originally classified ashaving predominantly neuronal properties (Schubert et al., 1974),B103 cells have consecutively been found to express appreciablelevels of mRNAs for several major myelin-specific proteins (Monukiet al., 1989). We also note the absence of endogenous Sox10 messagein U138 and COS7 cells, the two cell lines used in this studyfor transfection analyses (Fig. 3A; data not shown).

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Figure 3. Expression of Sox10 in cultured cells. A, Total cellular RNA from Schwann cells (SC) and several cell lines was analyzed forthe expression of Sox10 mRNA by Northern blot. Cell lines includedNB4 1A3 mouse neuroblastoma, N1E-115 mouse neuroblastoma, 3T3mouse fibroblasts, Rat1 fibroblasts, Neuro2A mouse neuroblastoma,C6 rat glioma, B103 rat tumor cells, 33B rat oligodendroglioma,HJC hamster glioma, P19 mouse embryonal carcinoma, and U138 humanglioblastoma. Filters were hybridized consecutively with probesspecific for Sox10 (top panel) and GAPDH (bottom panel). B, Totalcellular RNA from mature oligodendrocytes (OL) and CG-4 cellswas analyzed for the expression of Sox10 mRNA by Northern blot.CG-4 cells were either maintained in the undifferentiated state( $-$ ) or differentiated for various time intervals (1d-5d). Filterswere hybridized consecutively with probes specific for Sox10 (toppanel), MBP (middle panel), and GAPDH (bottom). C, Whole-cellextracts from purified rat Schwann cells (SC), primary oligodendrocyteprogenitors (O2-A) and mature oligodendrocytes (OL) were analyzedfor the presence of Sox10 protein by Western blot using a rabbitantiserum raised against Sox10 holoprotein.

Sox10 mRNA was strongly expressed in cultures of mature oligodendrocytes (Fig. 3B). To assess relative Sox10 expression duringdifferentiation of oligodendrocyte progenitors to mature oligodendrocytes,we took advantage of the CG-4 cell line (Louis et al., 1992).These cells provide a tissue culture model for oligodendrocytedifferentiation, because they resemble oligodendrocyte progenitorswhen cultured in the presence of PDGF and bFGF and because theycan be induced to differentiate by removal of growth factors (Louiset al., 1992; Sock et al., 1997), as judged from an increase inMBP levels (Fig. 3B). Sox10 mRNA levels remained high at all timesduring the differentiation process and did not change significantly.

To investigate whether the presence of Sox10 mRNA would be equalled by the presence of Sox10 protein, we performed Westernblot analysis on extracts from select cell types using the rabbitanti-Sox10 antiserum. A 56 kDa signal corresponding to Sox10 proteinwas not only detected in B103 and 33B cells (Fig. 1D) but alsoin primary Schwann cells, oligodendrocyte progenitors, and matureoligodendrocytes (Fig. 3C). Taken together, the data of Figures2 and 3 demonstrate that Sox10 is strongly expressed in the nervoussystem and can be preferentially detected in several glial celltypes or cell lines derived from them.

Expression pattern of Sox10 in the adult CNS

Expression of Sox10 transcripts in the adult CNS corresponded to a glial origin. Consistent with the previously establishedpresence of Sox10 in cultured oligodendrocytes (Fig. 3B), prominenthybridization was observed in all areas of the brain with a highcontent of myelinated fibers as the corpus callosum, the fimbria,the internal and external capsule, the anterior commissure, thestria medullaris of the thalamus (Fig. 4A), and the neuropil regionof the cerebellum (Fig. 4F). In other areas of the CNS hybridizationsignals were less intense. Emulsion autoradiography under high-powermagnification revealed that these latter signals were not causedby a weak, uniform labeling of all resident cells but insteadresulted from a lower density of strongly labeled cells. In thecerebral cortex, these cells were evenly distributed throughoutall layers (Fig. 4A-C). In the hippocampal formation and the cerebellum,scattered Sox10-positive cells were detected in the molecularlayer (Fig. 4A,D-G).

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Figure 4. Localization of Sox10 transcripts in adult and developing rodent brain. A, In situ hybridization of a frontal section throughan adult rat brain. Identical results were obtained on sectionsof adult mouse brain. B-G, High-power photomicrographs showingdistribution of silver grains in the cerebral cortex (B, C), thehippocampal formation (D, E), and the cerebellar cortex (F, G).H, In situ hybridization of a coronal section through a P7 mousehead. I, J, High-power photomicrographs exhibiting accumulationof silver grains over the optic nerves in a coronal section througha P7 mouse head. K, L, Distribution of Sox10 transcripts in acoronal section through the medulla oblongata at E14.5. M, N,Coronal section of the telencephalon at E16.5. Photomicrographsfrom overviews were taken from autoradiograms. High-resolutionpictures are bright-field photomicrographs (left) and their correspondingdark-field photomicrographs (right). anc, Anterior commissure;CA1, pyramidal cells; cc, corpus callosum; ec, external capsule;fi, fimbria; gc, granular cells; gl, granular layer; Hil, hilusof the dentate gyrus; hyp, hypothalamus; ic, internal capsule;ml, molecular layer of the cerebellar cortex; Mol, molecular layerof the dentate gyrus; neu, neuropil; opt, optic nerve; sm, striamedullaris of the thalamus; sr, stratum radiatum; IV, fourth ventricleof the brain. All other Roman numerals mark cranial nerves andganglia: v, trigeminal ganglion; vii, facial ganglion.

Expression pattern of Sox10 in the developing CNS

We determined the spatial pattern of Sox10 expression during development in postimplantation embryos from E6.5 through E18.5and in postnatal mice up to P21 using in situ hybridization. Sox10transcripts were first detected on E8.5 (Fig. 5A,J,K). They werespecifically localized to a small area of the dorsal neural tubeand the edges of the neural plate adjacent to already closed areas(Fig. 5A). Sox10 expression was not detected in any other regionof the trunk neural tube at this time (Fig. 5J,K). The regionsthat exhibited strong labeling for Sox10 corresponded to areasfrom which the neural crest cells originate. After E10.5, thissignal had disappeared (Fig. 5B,C). Up to E12.5, expression inthe CNS was marginal, with only a few weakly labeled cells presentin the spinal cord (Fig. 5L,M) and the medulla oblongata (datanot shown). At E13.5 labeling intensity in the CNS had increased.Outgrowing and ingrowing nerves now also exhibited prominent hybridizationsignals, as seen for example in the olfactory bulb (B. Herbarthand M. Wegner, unpublished data). At E14.5 faint signals wereobserved in nearly all areas of the brain (Fig. 5F). In the spinalcord and the medulla oblongata heavily labeled cells were locatedadjacent to but not within the ventricular zones (Fig. 4K,L; datanot shown). Detection of Sox10-positive cells in the spinal cordand in the medulla oblongata furthermore correlated with the firstappearance of oligodendrocyte progenitors in these regions (Nolland Miller, 1993; Pringle and Richardson, 1993; Hardy and Friedrich,1996). Up to E16.5 signal intensity in the brain had increased,and prominently labeled cells were now also seen in the frontalbrain (Fig. 4M,N). The number of Sox10-expressing cells furtherincreased up to E18.5 (Fig. 5H), before the adult pattern emergedduring the early postnatal period with strong hybridization signalsoverlying the fiber tracts (Figs. 4H, 5H,I) and the central nervessuch as the optic nerve (Fig. 4I,J). Fainter signals were seenover most other areas of the brain (Fig. 4H). At no time duringdevelopment or in the adult did we detect Sox10 transcripts inbrain nuclei.

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Figure 5. Localization of Sox10 transcripts in the developing PNS. A-I, In situ hybridization of embryonic mice as whole mounts (A-E,from E8.5 to E12.5) or sagittal sections (F-I, from E14.5 to P0).A, B, Dorsal views; C-E, lateral views. The ventral surface inlateral views and sagittal sections is to the right; the dorsalsurface is to the left. Intense hybridization signals are detectedover all ganglia and their corresponding nerve fibers. The arrowin A marks the labeled cells in the already closed neural tube.The arrowhead in E points to a hybridization signal in the cortex,which was also seen with the sense probe but was never detectedusing in situ hybridization on sections. Also note that no otherhybridization signal was obtained with the sense probe. J, K,Corresponding bright- and dark-field photomicrographs of transversesection through E8.5 neural tube. L, M, Corresponding bright-and dark-field photomicrographs of cross-section through E11.5spinal cord and the adjacent dorsal root ganglia. N, High magnificationof the E11.5 embryo in D, showing hybridization over all facial-cranialganglia and their fiber tracts. O, High magnification of the lowerback region of the E12.5 embryo in E. Arrows point to some ofthe nerve fibers leaving the spinal cord area. P, Q, Correspondingbright- and dark-field photomicrographs of cross-section throughthe stomach of an E13.5 mouse. Transcripts were detected in theouter wall of the stomach. R, S, Corresponding bright- and dark-fieldphotomicrographs of sagittal section through E16.5 sympathetictrunk and the dorsal root ganglia. T, Bright-field photomicrographof E18.5 trigeminal ganglion with superimposed hybridization signalsfor Sox10 (orange) and SorLA (purple). Hybridization signals wereobtained from dark-field images of adjacent sagittal sectionsand assigned false colors by computer imaging. U, Magnificationof area boxed in T. b1, Branchial arch 1; b2, branchial arch 2;drg, dorsal root ganglion; N.man, nervus mandibularis; N.max,nervus maxillaris; N.oph, nervus ophtalmicus; ot, otic vesicle;sc, spinal cord; st, stomach; sub, submandibulary gland; sym,sympathethic trunk. Cranial nerves and ganglia are in Roman numerals:v, trigeminal; vii, facial; viii, acoustic; ix, glossopharyngeal;x, vagus.

Expression of Sox10 in the PNS

As already mentioned, the pattern of Sox10 expression during early nervous system development is consistent with its presencein the emerging neural crest. At present, it is uncertain whetherSox10 is expressed in all cells of the forming neural crest orin a subpopulation. However, as development continued, Sox10 becamepreferentially expressed in those neural crest derivatives thatparticipated in PNS formation and was undetectable in other neuralcrest derivatives such as the facial-cranial mesoderm (Fig. 5B-E,N).

As demonstrated in Figure 5A-C, all ganglia of the PNS exhibited hybridization signals as soon as they formed. In these ganglia,neurons might either be derived from the neural crest (as in thedorsal root ganglia; Fig. 5, drg) or from the neural placodes(as in the cochlear-vestibular ganglion; Fig. 5, vii/viii). Incontrast, glial cells in peripheral ganglia always originate fromthe neural crest (LeDouarin, 1982). At E9.5, the dorsal root gangliaas well as the trigeminal and the cochlear-vestibular ganglionalready exhibited prominent hybridization signals (Fig. 5B). Thus,Sox10 expression in these ganglia was independent of the genealogyof their neuronal constituents. Additionally, hybridization signalsfor Sox10 and the neuronal marker SorLA (Hermans-Borgmeyer etal., 1997; Mörwald et al., 1997) were nonoverlapping in the developingtrigeminal ganglion (shown for E18.5 in Fig. 5T,U). From E10.5onward, nerve fibers were also marked by hybridization signals(Fig. 5C-E,N,O,R,S). This was especially obvious in the branchesof the trigeminal nerve and the sympathetic trunk (Fig. 5N,R,S).Labeling was not restricted to those fibers that originated inganglia but was also observed for fibers with a CNS origin. Theaxons of motor neurons were, for example, labeled over the wholelength up to their targets (Fig. 5O). Sox10 expression in gangliaand in nerves was maintained up to P21 and was also observed inthe adult for the sciatic nerve (Herbarth and Wegner, unpublisheddata). Hybridization signals were also detected in the entericnervous system (Fig. 5P,Q). In contrast to the expression in sensoryand sympathetic ganglia, these signals decreased with ongoingdevelopment.

Outside of the CNS and the PNS some glandular tissues exhibited hybridization signals (for example, the submandibulary glandin Fig. 5H,I). At this point it is uncertain whether this signalis derived from innervating nerve fibers or the glandular tissueproper.

Sox10 as transcriptional activator

The transcriptional activity of Sox proteins differs dramatically (van de Wetering et al., 1993; Kamachi et al., 1995; Yuanet al., 1995; Südbeck et al., 1996; Bell et al., 1997; Lefebvreet al., 1997). Some only exhibit transcriptional activity in combinationwith other transcription factors (Kamachi et al., 1995; Yuan etal., 1995). Thus, it was interesting to analyze how Sox10 wouldbehave when tested for its activity as a transcription factor.

Most Sox proteins recognize the motif 5 $'$ -AACAAAG-3 $'$ or its complement 5 $'$ -CTTTGTT-3 $'$ (van de Wetering et al., 1993). We testedbinding of Sox10 to an oligonucleotide containing this sequencein electrophoretic mobility shift assays (Fig. 6A). A fusion proteinbetween the HMG domain of Sox10 and GST avidly bound to this site,whereas no binding could be detected for the POU domain proteinTst-1/Oct6/SCIP. Changing the 5 $'$ -AACAAAG-3 $'$ motif to 5 $'$ -GGCAAAG-3 $'$ effectively abolished binding of Sox10 (data not shown), as observedpreviously for other Sox proteins (van de Wetering et al., 1993).

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Figure 6. Functional characterization of Sox10. A, Purified Sox10-GST protein (Sox10) and nuclear extracts from COS cells transfectedwith Tst-1/Oct6/SCIP (Tst-1) were analyzed in electrophoreticmobility shift assays for their ability to bind to a radiolabeledoligonucleotide (SX, sequence as shown) that contained a consensusbinding site for Sox proteins (van de Wetering et al., 1993).B, The Sox-responsive luciferase reporter plasmid 3xSX luc wastransfected into U138 glioblastoma cells in combination with emptyCMV expression plasmid ( $-$ ), pCMV/Sox4 (2 µg/plate; Sox4), pCMV/Sox10(2 µg/plate; Sox10), and pCMV/Tst-1 (2 µg/plate; Tst-1) as indicated.Luciferase activities were determined in three independent experiments,each performed in duplicate. Values from transfections with luciferasereporter and empty expression plasmid were arbitrarily set to1. Data from all other transfections are presented as fold inductionabove this level. C, The Gal4-responsive luciferase reporter (3xUASluc) was transfected into U138 glioblastoma cells together withexpression plasmids for the Gal4 DNA-binding domain (Gal4) orfor various Gal4 fusions (2 µg each). In addition to the Gal4DNA-binding domain, fusions contained full-length Sox10 (Gal4-Sox10),amino acids 1-101 of Sox10 (Gal4-Sox10 N), amino acids 181-466of Sox10 (Gal4-Sox10 C), or amino acids 1-240 of Tst-1/Oct6/SCIP(Gal4-Tst-1 N). Luciferase activities were determined in threeindependent experiments, each performed in duplicate. Data arepresented for each Gal4 fusion as fold induction above the levelof luciferase activity obtained in transfections with an expressionplasmid for the Gal4 DNA-binding domain, which was given an arbitraryvalue of 1. D, Expression of Gal4 fusion proteins in transfectedcells was confirmed by Western blot analyses of whole-cell extractsusing a monoclonal antibody against the Gal4 DNA-binding domain.Numbers on the left indicate sizes of molecular weight markersin kilodaltons.

Placement of this Sox binding site in front of a minimal promoter enables Sox10 to bind to this promoter. If Sox10 were atranscriptional activator, it should be capable of stimulatingsuch a promoter in transient transfections. However, no activationwas observed when we transfected a corresponding luciferase reporterconstruct in U138 cells together with Sox10, although other Soxproteins such as Sox4 effectively activated this reporter (Fig.6B). Additional attempts to detect transcriptional activity forSox10 proved equally unsuccessful. These included changes in thenumber of Sox binding sites within the promoter, substitutionof sequences flanking the Sox binding sites, and use of differentcell lines for transfection (data not shown).

In an independent assay, we screened for the presence of a modular transactivation domain within Sox10 by fusing various partsof Sox10 to the DNA-binding domain of Gal4 (Gal4-DBD). Transferof a heterologous transactivation domain to Gal4-DBD has beenshown to lead to the reconstitution of a functional transcriptionfactor and results in the activation of promoters with Gal4 bindingsites in transient transfections. This activation is best observedon combinations of Gal4 binding sites and a minimal promoter.Using such a promoter, a 32-fold stimulation was observed whena region corresponding to the N-terminal 240 residues of Tst-1/Oct6/SCIPwas transferred to Gal4-DBD (Fig. 6C). This region contains thetransactivation domain of Tst-1/Oct6/SCIP (Meijer et al., 1992;Monuki et al., 1993). In marked contrast, transfer of holo-Sox10to Gal4-DBD or of regions corresponding to amino acids 1-101 andamino acids 181-466, respectively, did not result in the activationof the Gal4-responsive promoter. Thus, neither holo-Sox10, northe region preceding the HMG-domain, nor the one behind it containeda detectable transactivation function despite the fact that allGal4/Sox10 fusion proteins were produced to similar levels intransfected cells as the isolated Gal4 DNA-binding domain or itsfusion with Tst-1/Oct6/SCIP (Fig. 6D).

A thymidine kinase promoter with added Gal4 binding sites also allowed us to probe for repressor domains within Sox10, becausethis particular promoter has a high basal activity and is sensitiveto repression by Gal4 fusion proteins. Neither the region N-terminalnor the region C-terminal to the HMG domain led to a more thantwofold reduction of promoter activity when fused to Gal4-DBD,arguing against the presence of a strong repressor domain withinSox10 (data not shown).

Sox10 as modulator of Tst-1/Oct6/SCIP function

Having failed to detect an autonomous transactivation function for Sox10, we asked whether Sox10 could function in combinationwith other transcription factors. Tst-1/Oct6/SCIP was a plausiblechoice, because both proteins are coexpressed during certain developmentalstages in several glial lineages (Monuki et al., 1990; Collariniet al., 1992), and because synergy had been shown between anotherpair of Sox and POU domain proteins (Yuan et al., 1995). Becauseno target gene for either Tst-1/Oct6/SCIP or Sox10 is known inglial cells, we used a promoter that in addition to the $beta$ -globinTATA box contained three copies of the FXO element. This elementhad been identified from the FGF-4 enhancer as a region that boundboth Sox2 and Oct-3/4 and thereby mediated the synergistic actionof both proteins in embryonic stem cells (Yuan et al., 1995).When Sox10 was transfected in U138 cells with a luciferase reportercontaining FXO elements, no changes in promoter activity wereobserved, further supporting our conclusion that Sox10 is nota strong transcription factor by itself (Fig. 7A). Transfectionof high amounts of Tst-1/Oct6/SCIP expression plasmid, on theother hand, led to a robust 11-fold stimulation of the same luciferasereporter. When both Sox10 and Tst-1/Oct6/SCIP were present, promoteractivity increased on average 29-fold above background levels,clearly indicating that Sox10 and Tst-1/Oct6/SCIP functioned synergisticallyin transfected cells. When less Tst-1/Oct6/SCIP expression plasmidwas used, so that promoter stimulation remained submaximal, westill detected a substantial increase in promoter activity withcotransfection of Sox10 (13- vs 5-fold in Fig. 7A). Synergisticactivation of this promoter by Tst-1/Oct6/SCIP and Sox10 was quantitativelysimilar to its activation by Oct-3/4 and Sox2, as evident bothfrom our transient transfections (Fig. 7A) and from the literature(Yuan et al., 1995).

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Figure 7. Synergistic action of Sox10 and POU domain proteins. A, The luciferase reporter plasmid 3xFXO luc was transfected into U138glioblastoma cells in combination with empty CMV expression plasmid( $-$ ), pCMV/Sox2 (0.2 µg/plate; Sox2), pCMV/Oct-3/4 (0.2 µg/plate;Oct-3/4), pCMV/Sox10 (0.2 µg/plate; Sox10), and pCMV/Tst-1 (0.2µg/plate; Tst-1; or 2 µg/plate, Tst-1) as indicated. Luciferaseactivities were determined in three independent experiments, eachperformed in duplicate. Values from transfections with luciferasereporter and empty expression plasmid were arbitrarily set to1. Data for all other transfections are presented as fold inductionabove this level. B, Radiolabeled FXO oligonucleotide with adjacentSox and POU domain binding sites (sequence as shown) was incubatedin electrophoretic mobility shift assays with purified recombinantSox10-GST (Sox10) and nuclear extracts from COS cells transfectedwith Tst-1/Oct6/SCIP (Tst-1) or Brn-1 (Brn-1). Antibodies (Ab)directed against Tst-1 (T), Brn-1 (B), or the GST portion of Sox10-GST(Sx) were added to the reactions as indicated below the lanes.Specific complexes between a protein and an FXO are marked bythe name of the respective protein, whereas the ternary complexof Sox10, POU domain protein, and DNA is labeled TC. The supershiftedcomplexes are marked by asterisks. C, The luciferase reporterplasmid 3xFXO luc was transfected into U138 glioblastoma cellsin combination with empty CMV expression plasmid ( $-$ ), pCMV/Sox10(0.2 µg/plate; Sox10), pCMV/Brn-1 (2 µg/plate; Brn-1), and pCMV/Brn-3.0(2 µg/plate; Brn-3) as indicated. Luciferase activities were determinedin three independent experiments and are presented as in A.

Using electrophoretic mobility shift assays, we subsequently assayed binding of both proteins to FXO (Fig. 7B). Tst-1/Oct6/SCIPas well as the previously described Sox10-GST fusion protein boundwith high affinity, each yielding a protein-DNA complex of characteristicmobility. When both proteins were simultaneously incubated withFXO, a third complex appeared that exhibited a significantly lowermobility than either the Sox10-FXO or the Tst-1/Oct6/SCIP-FXOcomplex. The presence of both Sox10 and Tst-1/Oct6/SCIP withinthis new complex was shown by antibody perturbation experiments.Addition of a Tst-1/Oct6/SCIP-specific antiserum led to the disruptionof both the Tst-1/Oct6/SCIP-FXO complex and the new complex butleft the Sox10-FXO complex intact. Incubation with antibodiesagainst the GST portion of the Sox10-GST fusion protein, on theother hand, resulted in the selective disappearance of the Sox10-FXOcomplex as well as the low-mobility complex with the concomitantformation of a supershifted complex. These results show conclusivelythat the low-mobility complex represents a ternary complex consistingof Tst-1/Oct6/SCIP, Sox10, and FXO. Ternary complex formationwas not favored over formation of binary complexes between FXOand either Tst-1/Oct6/SCIP or Sox10, making it unlikely that synergybetween both proteins is attributable to cooperative DNA binding.

Tst-1/Oct6/SCIP is highly related to a number of other POU domain proteins, including Brn-1 (Wegner et al., 1993; Ryan andRosenfeld, 1997). Because these proteins share very similar DNA-bindingcharacteristics, we were interested in studying whether otherPOU domain proteins could substitute functionally for Tst-1/Oct6/SCIP.When electrophoretic mobility shift analyses were performed withBrn-1 and Sox10 instead of Tst-1/Oct6/SCIP and Sox10, very similarresults were obtained (Fig. 7B). Importantly, Brn-1 was as effectivein forming a ternary complex with Sox10 and FXO as was Tst-1/Oct6/SCIP.

Despite similar binding characteristics, Brn-1 was, however, unable to stimulate transcription from an FXO-containing promotereither alone or in the presence of Sox10 (Fig. 7C). We also testedthe ability of Brn-3.0 (Gerrero et al., 1993) to function synergisticallywith Sox10. Again no significant increase in promoter activityabove the level of Brn-3.0 alone was detected on addition of Sox10,pointing to specificity in the interaction between Tst-1/Oct6/SCIPand Sox10.

In addition to FXO, which contained adjacent recognition sites for Sox and POU domain proteins, we also tested isolated Soxbinding sites for their ability to mediate synergy between Tst-1/Oct6/SCIPand Sox10. Figure 6 already showed that Tst-1/Oct6/SCIP was unableto bind to a Sox consensus binding site. Furthermore, Tst-1/Oct6/SCIPfailed to activate a promoter containing Sox binding sites eitherwhen present alone or in combination with Sox10. Thus, no synergywas observed between Tst-1/Oct6/SCIP and Sox10 when only Sox bindingsites were present in the promoter.

Using the reverse setup, we next tested whether a binding site for Tst-1/Oct6/SCIP would by itself be sufficient to confersynergistic activation by Tst-1/Oct6/SCIP and Sox10 on a minimalpromoter (Fig. 8). Sox10 neither activated a promoter that containedthree tandem copies of the octamer element from the HSV ICP0 gene,nor did it bind to this element in electrophoretic mobility shiftexperiments. Tst-1/Oct6/SCIP, on the other hand, stimulated thesame promoter sevenfold on average in transiently transfectedU138 cells (Fig. 8A), consistent with its ability to bind to theHSV octamer element in vitro (Fig. 8B). When Tst-1/Oct6/SCIP andSox10 were present during transfection, stimulation of the octamer-containingpromoter was comparable to rates achieved with Tst-1/Oct6/SCIPalone. This lack of cooperativity between both proteins on theHSV octamer element was also reflected by the absence of a ternarycomplex in electrophoretic mobility shift assays with this site.Thus, we conclude that both Sox10 and Tst-1/Oct6/SCIP have tobind independently to promoter DNA to function synergistically.

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Figure 8. Binding site requirements for cooperativity between Sox10 and Tst-1/Oct6/SCIP. A, The POU-responsive luciferase reporter plasmid3xHSVoct luc was transfected into U138 glioblastoma cells in combinationwith empty CMV expression plasmid ( $-$ ), pCMV/Sox10 (0.2 µg/plate;Sox10), and pCMV/Tst-1 (0.2 µg/plate; Tst-1) as indicated. Luciferaseactivities were determined in three independent experiments, eachperformed in duplicate. Values from transfections with luciferasereporter and empty expression plasmid were arbitrarily set to1. Data from all other transfections are presented as fold inductionabove this level. B, Purified Sox10-GST protein (Sox10) and nuclearextracts from COS cells transfected with Tst-1/Oct6/SCIP (Tst-1)were analyzed in electrophoretic mobility shift assays for theirability to bind to a radiolabeled HSVoct oligonucleotide, whichcontained the binding site for POU domain proteins from the HSVICP0 promoter, as shown at the top. The Tst-1/Oct6/SCIP-specificcomplex is marked by an arrowhead.

To identify the regions in Tst-1/Oct6/SCIP involved in synergistic action, we tested a series of Tst-1/Oct6/SCIP deletionmutants for their ability to cooperate with Sox10 (Fig. 9A). Thesemutants have been characterized previously and have been shownto be efficiently expressed and correctly localized to the nucleiof transfected cells (Renner et al., 1994; Sock et al., 1996a).As evident from Figure 9C, deletion of all amino acids C-terminalto the POU domain of Tst-1/Oct6/SCIP ( $Delta$ C mutant) did not interferewith synergistic activation of the FXO-containing promoter intransfected U138 cells. A Tst-1/Oct6/SCIP mutant devoid of thePOU-specific domain ( $Delta$ P_S mutant), on the other hand, was incapableof functionally interacting with Sox10. This might be expected,because removal of the POU-specific domain strongly reduces theability of Tst-1/Oct6/SCIP to interact with its binding site inFXO. Deletion of the region N-terminal to the POU domain of Tst-1/Oct6/SCIPlikewise abolished cooperativity with Sox10, indicating that theN-terminal region of Tst-1/Oct6/SCIP is involved in the observedsynergy. Similar results were obtained independent of whetherTst-1/Oct6/SCIP mutants were used in limiting amounts (Fig. 9C)or saturating amounts (data not shown).

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Figure 9. Protein domains involved in synergism between Sox10 and Tst-1/Oct6/SCIP. A, Summary of Tst-1/Oct6/SCIP and Sox10 mutants.Tst-1 $Delta$ N, Mutant Tst-1/Oct6/SCIP lacking amino acids 4-240; Tst-1 $Delta$ P_S,mutant Tst-1/Oct6/SCIP lacking amino acids 241-319; Tst-1 $Delta$ C, mutantTst-1/Oct6/SCIP lacking amino acids 396-448; Sox10 $Delta$ N, mutant Sox10lacking amino acids 1-89; Sox10HMG, comprising amino acids 101-180of Sox10. B, Comparison of expression levels between Sox10 andits mutants Sox10 $Delta$ N and Sox10HMG in nuclear extracts of transfectedcells by Western blot using rabbit antiserum against Sox10. Numberson the left indicate sizes of molecular weight markers in kilodaltons.C, D, The luciferase reporter plasmid 3xFXO luc was transfectedinto U138 glioblastoma cells in combination with empty CMV expressionplasmid ( $-$ ), pCMV/Sox10 (Sox10), pCMV/Tst-1 (Tst-1), and variousmutant versions of both plasmids (all 0.2 µg/plate) as indicated.Luciferase activities were determined in three independent experiments,each performed in duplicate. Values from transfections with luciferasereporter and empty expression plasmid were arbitrarily set to1. Data for all other transfections are presented as fold inductionabove this level.

To investigate which domains of Sox10 would be involved in the synergistic interaction, we also constructed several Sox10mutants (Fig. 9A). Sox10HMG represented the HMG domain of Sox10,whereas Sox10 $Delta$ N corresponded to a truncated Sox10 version withresidues 1-89 missing. All proteins were efficiently producedin transfected cells and similar to full-length Sox10 targetedto the nucleus, as judged from Western blot analyses of nuclearextracts from transfected cells (Fig. 9B). Despite their efficienttranslation, none of the mutant Sox proteins proved capable ofcooperative interaction with Tst-1/Oct6/SCIP (Fig. 9D). Thus,we conclude that the HMG domain is not sufficient to obtain synergy.A second region in the N-terminal part of Sox10 is additionallyrequired.

Sox10 as transcriptional modulator of other glial transcription factors

Sox10 is expressed in Schwann cells also at times when Tst-1/Oct6/SCIP is missing. Therefore, we speculated that Sox10 mighthave comparable modulatory function on other transcription factorsthat are expressed at stages of Schwann cell development duringwhich Tst-1/Oct6/SCIP is absent. The paired domain protein Pax3and the zinc finger protein Krox-20 have been characterized previouslyas such proteins (Blanchard et al., 1996; Zorick et al., 1996).To test the ability of Sox10 to interact functionally with eitherPax3 or Krox-20, we used promoters that contained adjacent bindingsites for one of these transcription factors and Sox proteins(Fig. 10A). The exact configuration of sites was modeled afterthe arrangement of Sox and POU domain binding sites in FXO.

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Figure 10. Synergistic interaction among Pax3, Krox-20, and Sox10. A, Arrangement of binding sites for Pax3, Krox-20, and Sox10 in theFXP and FXK oligonucleotides. B, The luciferase reporter plasmid3xFXP luc, which contained adjacent binding sites for Pax3 andSox10, was transfected into U138 glioblastoma cells in combinationwith empty CMV expression plasmid ( $-$ ), pCMV/Sox10 (0.2 µg/plate;Sox10), and pCMV/Pax3 (50 ng/plate; Pax3) as indicated. C, Theluciferase reporter plasmid 2xFXK luc, which contained adjacentbinding sites for Krox-20 and Sox10, was transfected into U138glioblastoma cells in combination with empty CMV expression plasmid( $-$ ), pCMV/Sox10 (0.2 µg/plate; Sox10), and pCMV/Krox-20 (50 ng/plate;Krox-20) as indicated. Luciferase activities were determined inthree independent experiments, each performed in duplicate. Valuesfrom transfections with luciferase reporter and empty expressionplasmid were arbitrarily set to 1. Data for all other transfectionsare presented as fold induction above this level.

When transient transfections were performed with a promoter construct containing adjacent Sox and Pax binding sites, no significantstimulation could be observed for either protein alone over awide range of concentrations (Fig. 10B; data not shown). Combinationof Sox10 with low amounts of Pax3, however, resulted in a strong12-fold stimulation of the promoter construct, indicating thatSox10 synergistically interacted with Pax3 in a manner similarto its interaction with Tst-1/Oct6/SCIP.

Results were different in transient transfections with a promoter construct in which Sox binding sites were placed next tobinding sites for Krox-20. This promoter did not respond to Sox10but in U138 cells was activated by Krox-20 even at low concentrations(Fig. 10C). This time, the presence of both Sox10 and Krox-20 intransfected cells led to a promoter stimulation significantlybelow the one obtained for Krox-20 alone (threefold compared withsevenfold). Thus, Sox10 seemed to repress Krox-20 function partiallyin the context of this particular promoter construct. Becausethis effect might be dependent on the spacing, orientation, andprecise sequence of binding sites for both transcription factors,different effects of Sox10 on Krox-20 (or Pax3) activity mightbe observed in the context of other promoters. This caveat notwithstanding,both Pax3 and Krox-20 were clearly modulated in their activityby the presence of Sox10.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Recent evidence suggests that proteins with similarity to the sex determining factor SRY are not only involved in varioussteps of gonadal development and spermatogenesis. These so-calledSox proteins also function as important transcriptional regulatorsin a variety of other developmental processes, including chondrogenesis,haemopoiesis, and neurogenesis (Pevny and Lovell-Badge, 1997).

For the first time, we now report the complete amino acid sequence of Sox10 from rat. Sox10 belongs to the same subgroup ofSox proteins as Sox9 and Sox8 (Wright et al., 1993; Pevny andLovell-Badge, 1997). Whereas expression pattern and function ofmammalian Sox8 are still unknown, Sox9 has been shown recentlyto be involved in chondrogenesis and male sex determination suchthat inactivation of Sox9 leads to campomelic dysplasia and autosomalsex reversal in human patients (Foster et al., 1994; Wagner etal., 1994; Wright et al., 1995; daSilva et al., 1996).

Despite sequence similarities, Sox10 exhibited a unique expression pattern among Sox proteins. Sox10 expression was firstdetected in the emerging neural crest. Later during developmentand in the adult, Sox10 was preferentially and abundantly expressedin glial cells. Evidence for a predominantly glial expressionof Sox10 in both PNS and CNS is manifold. For one, Sox10 transcriptand protein were detected in primary cultures of Schwann cellsand oligodendrocytes as well as in a number of cell lines derivedfrom glia. In the PNS, intense labeling could be detected notonly in ganglia but also along motor axons and sciatic and trigeminalnerves, as well as in the sympathetic trunk, implying that Sox10is expressed in Schwann cells. Furthermore, expression of Sox10in the adult CNS was prominent in areas with high nerve fibercontent and could be localized over myelinated fiber tracts suchas anterior commissure, corpus callosum, and fimbria. This patternand the presence of Sox10 in the optic and other central nervesare both strongly indicative of oligodendrocytic expression. Incontrast, Sox10-specific signals were not detected over brainnuclei, arguing against mainly neuronal expression. Even the presenceof scattered labeled cells in other areas of the brain was moreconsistent with Sox10 expression in glia than in neurons. Whereanalyzed, Sox10 expression did not exhibit significant overlapwith neuronal markers in peripheral ganglia or in the CNS (Herbarthand Wegner, unpublished data). Thus, Sox10 might turn out to bea valuable marker for future lineage studies of glial cells invivo.

The continued expression of Sox10 contrasts sharply with the transient expression of several other Sox proteins (Gubbay etal., 1990; Wright et al., 1995). Because of the transience oftheir expression, these proteins are thought to function as geneticswitches that determine the fate of precursor cells at a specificpoint in their development (Pevny and Lovell-Badge, 1997). Expressionof Sox10, in contrast, argues for a role of Sox10 in definingand maintaining the identity of the glial phenotype.

The expression of Sox10 also markedly differs from the expression pattern of transcription factors identified previously inglial cells, because these latter proteins are only present duringspecific developmental stages or in the mature glial cell (Monukiet al., 1990; Collarini et al., 1992; Topilko et al., 1994; Kioussiet al., 1995; Bermingham et al., 1996; Blanchard et al., 1996;Zorick et al., 1996; Sock et al., 1997). Furthermore, all of theother proteins are not only expressed in glia but additionallyin a variety of other cell types, so that Sox10 exhibits by farthe most restricted expression pattern.

What could be the function of Sox10 in glial cells? Our results indicate that Sox10 is not a strong transcriptional activatorby itself and most likely exerts its function in concert withother transcription factors. Because there is precedence for acombinatorial function of Sox and POU domain proteins from studieson embryonal stem cells (Yuan et al., 1995), we decided to lookfirst into the possibility of an interaction between Sox10 andTst-1/Oct6/SCIP, a POU domain protein shown to be present in Schwanncells and oligodendrocytes (Monuki et al., 1990; Collarini etal., 1992; Scherer et al., 1994; Blanchard et al., 1996; Zoricket al., 1996). Indeed, we were able to show that both proteinssynergistically activated transcription from a promoter that containedadjacent binding sites for Sox and POU domain proteins. Promoteractivation was as efficient for Tst-1/Oct6/SCIP and Sox10 as observedpreviously for Oct-3/4 and Sox2 (Yuan et al., 1995). Both Tst-1/Oct6/SCIPand Sox10 were required to bind to the promoter, as evident fromthe absence of synergistic action on promoters that containedonly Sox protein binding sites or binding sites for POU domainproteins. Binding of Sox10 and Tst-1/Oct6/SCIP to adjacent sitesin the promoter was visualized as a ternary complex of both proteinswith DNA in electrophoretic mobility shift assays. Despite beingan essential requirement for synergistic function, formation ofsuch a ternary complex was in itself not sufficient. This becameevident from the fact that Brn-1, a POU-domain protein relatedto Tst-1/Oct6/SCIP (He et al., 1989; Ryan and Rosenfeld, 1997),was unable to cooperate with Sox10 on a functional level despitebeing able to form Sox10-containing ternary complexes with efficienciessimilar to Tst-1/Oct6/SCIP. Comparable results were obtained inthe original study on synergy between Sox2 and Oct-3/4 on theFGF-4 promoter in which Oct-1 formed ternary complexes with Sox2but still could not substitute functionally for Oct-3/4 (Yuanet al., 1995).

The inability of both Brn-1 and Brn-3.0 to cooperate functionally with Sox10 lends further proof to the specificity of theinteraction between Sox10 and Tst-1/Oct6/SCIP. Given the factthat both the POU domain and the N-terminal part of Tst-1/Oct6/SCIPwere required for the interaction, it seems reasonable to assumethat it is mainly the N-terminal domain of Tst-1/Oct6/SCIP thatis responsible for this specificity, because this region is notconserved in other POU domain proteins (Wegner et al., 1993; Ryanand Rosenfeld, 1997).

An equally important finding of our study is that the HMG domain of Sox10 is not sufficient to mediate synergy with Tst-1/Oct6/SCIP.Thus, it is unlikely that the observed functional interactionbetween both proteins is simply attributable to the strong DNA-bendingcapacity intrinsic to proteins carrying an HMG domain (Giese etal., 1992). The requirement for the 89 N-terminal residues ofSox10 implies that if Sox10 exerts its function as an architecturalprotein and mediates assembly of nucleoprotein complexes on promoterDNA, it must do so not only by DNA bending but also through highlyspecific protein-protein interactions that presumably involveits N-terminal domain.

Whatever the mechanism, Sox10 is unlikely to function exclusively as a modulator of Tst-1/Oct6/SCIP function, because itsexpression starts long before the onset of Tst-1/Oct6/SCIP expressionand continues beyond it. We therefore postulated that Sox10 mightsimilarly influence the function of transcription factors activein other stages of glial development. Intriguingly, this was indeedthe case for Pax3 (Kioussi et al., 1995), which was synergisticallyactivated, and for Krox-20 (Topilko et al., 1994), which was partiallyrepressed when tested on a synthetic promoter construct. Althoughthe effect of Sox10 on transcription factors such as Pax3, Krox-20,and Tst-1/Oct6/SCIP will likely depend on the spacing, orientation,and precise sequence of binding sites for these transcriptionfactors in a promoter, our results clearly prove that Sox10 hasthe capacity to function as a glia-specific transcriptional modulator.A more detailed analysis of Sox10 function will have to awaitthe identification of genuine target genes for Sox10 in glialcells.

A cell-specific modulator has been postulated repeatedly for Tst-1/Oct6/SCIP to explain its preferential activity in glialcells (Monuki et al., 1993; Sock et al., 1996b). The existenceof such a modulator would have the additional advantage of beingable to confer strict cell specificity to the function of proteinsthat are preferentially, but not exclusively, expressed in a givencell, as is the case for Tst-1/Oct6/SCIP, Pax3, and Krox-20 (Topilkoet al., 1994; Kioussi et al., 1995; Bermingham et al., 1996).We therefore propose that transcription factors such as Tst-1/Oct6/SCIP,Pax3, and Krox-20 are able to regulate specific target genes inglial cells because of the presence of transcriptional modulatorssuch as Sox10. Different combinations of stage-specific transcriptionfactors with the same glia-specific modulator would thus mediatethe spatially and temporally unique gene activation events thatcatalyze glial development. Different modulators in other celltypes would also allow the same transcription factors to targetother genes in different cells, thus tailoring transcription factorfunction to the need of the cell.

  FOOTNOTES

Received Aug. 6, 1997; revised Oct. 1, 1997; accepted Oct. 22, 1997.

This work was supported by Deutsche Forschungsgemeinschaft Grant We1326/5-2 to M.W. We thank P. Matthias, J. C. Louis, andR. Lovell-Badge for providing reagents. H. C. Schaller is acknowledgedfor generously allowing us to use the equipment of her institute.Daniela Feist and Birgitta Schinke provided expert technical assistance.
Correspondence should be addressed to Michael Wegner, Zentrum für Molekulare Neurobiologie, Martinistrasse 52, D-20246 Hamburg,Germany.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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