Functional Interactions between Drosophila bHLH/PAS, Sox, and POU Transcription Factors Regulate CNS Midline Expression of the slit Gene

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The Journal of Neuroscience, June 15, 2000, 20(12):4596-4605

Functional Interactions between Drosophila bHLH/PAS, Sox, and POU Transcription Factors Regulate CNS Midline Expression of the slit Gene
Yue Ma¹, Kaan Certel², Yanping Gao¹, Emily Niemitz¹, Jack Mosher³, Ashim Mukherjee¹, Mousumi Mutsuddi¹, Neda Huseinovic¹, Stephen T. Crews³, Wayne A. Johnson², and John R. Nambu¹
¹ Department of Biology, University of Massachusetts, Amherst, Massachusetts 01003, ² Genetics Ph.D. Program and Department of Physiology and Biophysics, University of Iowa, Iowa City, Iowa 52242, and ³ Department of Biochemistry and Biophysics, School of Medicine, University of North Carolina, Chapel Hill, North Carolina 27599

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

During Drosophila embryogenesis the CNS midline cells have organizing activities that are required for proper elaborationof the axon scaffold and differentiation of neighboring neuroectodermaland mesodermal cells. CNS midline development is dependent onSingle-minded (Sim), a basic-helix-loop-helix (bHLH)-PAS transcriptionfactor. We show here that Fish-hook (Fish), a Sox HMG domain protein,and Drifter (Dfr), a POU domain protein, act in concert with Single-mindedto control midline gene expression. single-minded, fish-hook,and drifter are all expressed in developing midline cells, andboth loss- and gain-of-function assays revealed genetic interactionsbetween these genes. The corresponding proteins bind to DNA sitespresent in a 1 kb midline enhancer from the slit gene and regulatethe activity of this enhancer in cultured Drosophila Schneiderline 2 cells. Fish-hook directly associates with the PAS domainof Single-minded and the POU domain of Drifter; the three proteinscan together form a ternary complex in yeast. In addition, Fishcan form homodimers and also associates with other bHLH-PAS andPOU proteins. These results indicate that midline gene regulationinvolves the coordinate functions of three distinct types of transcriptionfactors. Functional interactions between members of these proteinfamilies may be important for numerous developmental and physiologicalprocesses.

Key words: Drosophila; CNS midline; bHLH/PAS; Sox; POU; slit; gene expression

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

During Drosophila embryogenesis, a group of specialized CNS midline neurons and glia provide signals that are essential forthe differentiation of neighboring ectodermal and mesodermal cells(for review, see Crews, 1998). The CNS midline also serves asan intermediate axon guidance target that expresses chemotacticfactors, including Slit, Commissureless, and D-Netrin, which controlaxon crossing at the midline (Harris et al., 1996; Mitchell etal., 1996; Tear et al., 1996; Kidd et al., 1999). In particular,Slit is a conserved epidermal growth factor (EGF)-repeat proteinthat is strongly expressed by midline glia and interacts withthe Roundabout receptor to prevent commissural axons from recrossingthe midline (for review, see Guthrie, 1999; Van Vactor and Flanagan,1999; Zinn and Sun, 1999). Development of the entire CNS midlinelineage requires the gene regulatory functions of Single-minded(Sim), a basic-helix-loop-helix (bHLH)-PAS transcription factor(Nambu et al., 1991). Sim protein forms functional heterodimerswith Tango (Tgo), a bHLH-PAS protein that exhibits widespreadembryonic expression (Sonnenfeld et al., 1997; Ward et al., 1998).Sim:: Tgo heterodimers act through the CNS midline element (CME),an ACGTG sequence motif present in the regulatory regions of slitand other midline-expressed genes (Wharton et al., 1994; Sonnenfeldet al., 1997; Kasai et al., 1998). A CME present in a 380 bp slitregulatory DNA fragment is essential for midline expression ofa linked reporter gene (Wharton et al., 1994), although sequencesin addition to the CME are required for high levels of gene expression(Wharton and Crews, 1993). Interestingly, results from Sim ectopicexpression experiments suggest that in addition to Tgo, Sim functionallyinteracts with other factors more specifically expressed in themidline and lateral and cephalic neuroectoderm (Nambu et al.,1991; Muralidhar et al., 1993).

One candidate for such a Sim cofactor is the Sox HMG domain protein Fish-hook (Fish) (Nambu and Nambu, 1996; Russell et al.,1996). Fish is strongly expressed in the early neuroectoderm andis required for proper differentiation of midline and lateralCNS cells (Nambu and Nambu, 1996; Ma et al., 1998; Sánchez Sorianoand Russell, 1998). The Fish HMG domain binds DNA sequences relatedto AACAAT and AACAAAG and induces strong DNA bending (Ma et al.,1998). This suggests that Fish may provide chromatin architecturalfunctions to facilitate the assembly of higher-order protein/DNAcomplexes. In this regard, the closely related vertebrate Sox2protein directly associates with the Oct3 POU domain protein tosynergistically activate expression of the fgf4 gene (Yuan etal., 1995; Ambrosetti et al., 1997). fish mutants exhibit geneticinteractions with mutations in Drosophila POU genes (Ma et al.,1998; Sánchez Soriano and Russell 1998), and one of these POUgenes, drifter (dfr), is expressed in the CNS midline and is essentialfor proper midline glial migrations (Anderson et al., 1995).

In this study we use genetic, biochemical, and cell culture assays to show that Sim, Fish, and Drifter (Dfr) act togetherto regulate CNS midline development and gene expression. In particular,these proteins synergistically influence slit transcription byacting through a 1 kb midline regulatory region that containsa single CME, as well as binding sites for Fish and Dfr. Regulationof slit expression appears to involve direct interactions betweenFish, Sim, and Dfr. Fish directly associates with the Sim PASdomain and the Dfr POU domain, and the three proteins can forma ternary complex in yeast cells. These results identify novelregulatory interactions between bHLH-PAS, Sox, and POUproteins.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fly strains. The following strains were used in this study: the fish⁸⁷ null mutant (Nambu and Nambu, 1996), the dfr^E82 lethal mutant (Anderson et al., 1995), P[1.0slit-lacZ] (Nambuet al., 1991; Wharton et al., 1994), P[UAS-fish] (Mukherjee etal., 2000), P[UAS-sim] (Xiao et al., 1996), and P[GMR-Gal4] (obtainedfrom the Bloomington Drosophila Stock Center (Bloomington, IN);generated by M. Freeman). A dfr^E82-fish⁸⁷/TM3, P[ftz-lacZ] strain was generated via meioticrecombination.

Immunostaining of Drosophila embryos. For single-label immunostaining experiments, embryos were collected from wild-type andmutant strains, as well as from genetic crosses, and fixed inPEM buffer (0.1 M PIPES, pH 6.9, 2 mM EGTA, 1 mM MgSO₄) with 4%formaldehyde (Patel, 1994). The embryos were incubated overnightwith primary antibodies in PTN (1× PBS, 0.2% Triton X-100, 5%normal horse serum). Vectastain biotinylated secondary antibodiesand streptavidin/horseradish peroxidase reagents (Vector Laboratories,Burlingame, CA) were used with H₂0₂/diaminobenzedine histochemistryto detect primary antibody binding. The monoclonal antibody (mAb)BP102 (Developmental Studies Hybridoma Bank, Iowa City, IA) wasused at a 1:4 dilution. A monoclonal antibody against $beta$ -galactosidase( $beta$ -Gal) (Promega, Madison, WI) was used at a 1:500 dilution. Stainedembryos were dehydrated through an ethanol series, mounted inmethyl salicylate and Permount (Fisher), and examined via Nomarskioptics using a Nikon Optiphot compoundmicroscope.

For double-label fluorescence immunostaining experiments, embryos were fixed in PEM buffer with 4% formaldehyde. They werelabeled by following previously described protocols (Mitchisonand Sedat, 1983; Johnson, 1992). $beta$ -Gal expression was detectedusing either a rabbit polyclonal antiserum (Cappel, West Chester,PA) at a 1:500 dilution or a mouse mAb 40-1a (Developmental StudiesHybridoma Bank) at a 1:3 dilution. Pre-absorbed rat anti-Dfr serumwas used at a final dilution of 1:3000 and rabbit anti-Fish serumat a dilution of 1:1000. After repeated washes in PBT (1× PBS,0.5% bovine serum albumin, 0.2% Triton X-100), embryos were incubatedwith FITC-conjugated anti-rat (Jackson ImmunoResearch Laboratories,West Grove, PA) and rhodamine-conjugated anti-mouse (Jackson ImmunoResearchLaboratories) or anti-rabbit (Biosource, Camarillo, CA) secondaryantibodies at 1:200 dilution. Stained embryos were mounted inVectashield (Vector Laboratories) and observed using a Bio-RadMRC-1024 confocalmicroscope.

DNA sequence analysis. DNA sequencing of the slit 1 kb midline regulatory region was performed by Retrogen, Inc. (San Diego,CA). The DNA fragment was sequenced by primer walking approaches,and the sequences from both strands were obtained in multipleruns. The analysis revealed this fragment to be 970 bp in lengthand flanked by two HinDIIIsites.

Gel mobility shift assays. For Fish gel mobility shift assays, two sets of complementary 26 mer oligonucleotides correspondingto Sox consensus DNA binding sites from the slit regulatory fragmentwere synthesized and annealed in 1× T4 polynucleotide kinase buffer(Promega). The sequence of the upper strand of each pair of oligonucleotidesis shown below, and the underlined sequence corresponds to Soxconsensus DNA binding sites (see Fig. 4A for location of probesequences): TACAAT probe $---$ 5'-ACTATACTATATTGTATTATGCACAG-3'; TTCAATprobe $---$ 5'-ACTGTATTCAATTTCATTGAAACAAA-3'.

The annealed oligonucleotides were end-labeled using T4 polynucleotide kinase (Life Technologies, Gaithersburg, MD) and $gamma$ -³²P-ATP (New England Nuclear) and gel-purified. Gel mobility shiftassays were performed using a purified 6XHis-HMG Fish fusion proteinas described previously (Ma et al., 1998).

For Dfr gel mobility shift assays, probes were generated by end-labeling double stranded oligonucleotides with $gamma$ -³²P-ATP (ICN Biochemicals, Costa Mesa, CA) and T4 polynucleotidekinase (New England Biolabs). The sequence of the upper strandsof each pair of oligonucleotides is shown below, and the underlinedsequence corresponds to consensus Dfr binding sites (see Fig.4A for location of probe sequences): ATGCAAAT probe $---$ 5'-ATGCACGACATATTTGCATTTTAAAATAGAGAA-3';CATAAAT probe $---$ 5'-ATATATGTCCCATTTATGTG- AGTGACATTCCA-3'.

Full-length Dfr protein was expressed in bacteria as a glutathione-S-transferase (GST) fusion protein and purified over glutathione-Sepharosebeads (Amersham Pharmacia, Arlington Heights, IL) as previouslydescribed (Certel et al., 1996). While on beads, the GST affinitytail was cleaved by using PreScission protease (Amersham Pharmacia)as per manufacturer's suggestions. End-labeled probes were incubatedwith full-length Dfr protein at room temperature for 15 min inbinding buffer (25 mM HEPES, pH 7.6, 12.5 mM MgCl2, 0.1 mM EDTA,100 mM KCl, 10% glycerol, 1 mM DTT). Immediately after incubation,the complexes were resolved on 5% native polyacrylamide gels atroom temperature in 1× TBE buffer. Gels were dried and exposedto Kodak X-OMATfilm.

Yeast two-hybrid assays. The yeast two-hybrid vectors pEG202 and pJG4-5 (Origene) were used to generate bait and prey constructs.Baits contained the LexA DNA binding domain fused to the proteinof interest, and the prey contained fusions to the B42 transcriptionalactivation domain. A chromosomally integrated LexAop-LEU2 reportergene was used that contains six LexA operator sites fused to theLEU2 gene. The bait and prey constructs were cotransformed intoEGY48 host yeast cells (Mat $alpha$ trp1 his3 ura3 leu2:: :6lexAop-LEU2)according to the supplier's instructions (Origene). The transformedcells were plated on YNB/Leu/Ura (-His, -Trp) glucose medium andincubated at 30°C for 3-4 d. Resulting transformants were thenplated on the YNB/Ura (-His, -Leu, -Trp) galactose/raffinose mediumand incubated at 30°C for 3-7 d to assay for the presence of coloniesthat indicatedinteractions.

Bait constructs that express full-length Fish, or truncated versions consisting of the N-terminal 141 amino acids, the 79amino acid HMG domain, the COOH-terminal 164 amino acids, theNH₂+HMG, the HMG+COOH, and the NH₂+COOH, are described in Ma etal. (1998). To generate a full-length Fish prey construct, theentire Fish 382 amino acid open reading frame was amplified viaPCR from full-length fish cDNA clone 2-5 (Nambu and Nambu, 1996)using the following primers: 5'-AGAGAATTCATGGCCACCTTATCGACACACCC-3';5'-TGTGAATTCCTACTAATAGAGCACCGGAACCGGTCGCCT-3'.

The resulting DNA fragment was digested with EcoRI, purified via agarose gel electrophoresis, and cloned into the pJG4-5vector.

Prey constructs that express full-length Dfr or the Dfr POU domain were generated via PCR using a full-length dfr p128 cDNAclone (Anderson et al., 1995) and the following primers: full-lengthDfr $---$ 5'-CATGGAATTCCCCACGTCCGATGATCTGGAGGCC-3', 5'-CATGCTCGAGTTACTAGTGGGCCGCCAACTGATGCGCCGC-3';Dfr POU domain (amino acids 210-362) $---$ 5'-CCCCGAATTCACGTCCGATGATCTGGAGGCC-3',5'-GGGGCTCGAGCGTCATGCGCTTCTCCTTCTG-3'.

The PCR products were digested with EcoRI and XhoI, purified via agarose gel electrophoresis, and subcloned into the pJG4-5vector.

A prey construct expressing the POU domain of Pdm-1 (amino acids 420-601) was generated via PCR from the full-length C616AcDNA clone (Billin et al., 1991), kindly provided by Steve Poole(University of California Santa Barbara), and the following primers:5'- CATGGAA-TTCCCGGAGGAAACCACCGATCTAGAA-3'; 5'-CATGCT CGA- GTTACTAGGGACTGTCCAGGG-AGGGATTGAT-3'.

A similar pdm-2 POU domain (amino acids 283-457) prey construct was generated via PCR from the full-length C9A cDNA clone(Billin et al., 1991) and the following primers: 5'- CATGGAATTCGAACAATCGCCGGAAGAGACCACC-3';5'-CATGCTCGAGTTACTAGTCCAGATCCAGCGAGGGATTGAT-3'.

Both pdm-1 and pdm-2 PCR products were digested with EcoRI and XhoI, purified via agarose gel electrophoresis, and subclonedinto the pJG4-5vector.

A prey construct that expresses the full-length mouse Oct3 protein was generated via PCR from a full-length pGEX-2-Oct3 cDNAclone, kindly provided by Lisa Dailey (New York University) (Yuanet al., 1995), and the following primers: 5'-GGGGAATTCATGTTCGAGAAGGTGGAACCAA-3';5'-GGGCTCGAGTCACCCTGTAGCCTCATACT- CTT-3'.

The PCR product was digested with EcoRI and XhoI, purified via agarose gel electrophoresis, and subcloned into the pJG4-5vector.

The following Sim and Trachealess (Trh) bait or prey constructs (in the pEG202 and pJG4-5 vectors) were used: full-lengthSim (amino acids 1-673), Sim bHLH-PAS (amino acids 1-461), SimbHLH-PAS-A (amino acids 1-183), Sim bHLH (amino acids 1-92), SimPAS (amino acids 58-370), full-length Trh (amino acids 1-929),and Trh bHLH-PAS (amino acids 1-689) (Sonnenfeld et al., 1997;M. Sonnenfeld and S. T. Crews, unpublished results). The Period(Per) bait (Per-C2) construct containing the PAS domain and aCOOH-extended region (amino acids 233-685) was kindly providedby Michael Rosbash (Brandeis University) (Huang et al., 1995).

To express native full-length Fish protein in yeast, the entire Fish open reading frame was amplified via PCR from fish cDNAclone 2-5 using the following primers: 5'-GGGGGAAGCTTATGGCCACCTTATCGACA-3';5'-CCCCCAAGCTTCTAATAGAGGACCGGAAC-3'.

The resulting DNA fragment was digested with HindIII, purified via agarose gel electrophoresis, and cloned into the pDB-20yeast expression vector (Becker et al., 1991). pDB20 permits highlevel of transgene expression driven by the ADC1 (ADH1) promoterand contains the selectable URA3marker.

To analyze interactions between Fish, Sim, and Dfr, full-length Sim bait, full-length Dfr prey, and full-length native Fishconstructs were transformed into EGY48 host cells. The cells weregrown on YNB/Leu (-His, -Ura, -Trp) glucose plates and incubatedat 30°C for 3-4 d. Transformed colonies were then streaked onYNB (-His, -Leu, -Trp, -Ura) galactose/raffinose plates and incubatedat 30°C for 4 d. For controls, full-length Sim bait and nativeFish or full-length Dfr prey and native Fish constructs were transformedinto EGY48 cells that were grown on YNB/Trp/Leu (-His, -Ura) glucoseplates at 30°C for 3-4 d. Transformed colonies were then streakedon the YNB/His (-Leu, -Trp, -Ura) or YNB/Trp (-His, -Leu, -Ura)galactose/raffinose plates and incubated at 30°C for 4d.

GST pulldown assays. Full-length ³⁵S-labeled Sim protein was generated from sim cDNA clone F1 (Nambu et al., 1991) using anin vitro transcription/translation reaction (Promega) and ³⁵S-methionine (Amersham Pharmacia). For the GST-Fish fusion protein,a DNA fragment encoding the full-length Fish protein, was generatedby PCR using fish cDNA clone 2-5 as a template and the followingtwo oligonucleotide primers: 5'-GGCCGAATTCATGCCACCTTATCGACACACCCCAAT-3';5'-CCGGGAATTCTTACTAATAGAGCACCGGAACCGG-3'.

The resulting PCR product was digested with EcoRI, purified via agarose gel electrophoresis, and subcloned into the pGEX-2Tvector (Amersham Pharmacia) to generate an in-frame fusion withGST. The resulting construct was transformed into Escherichiacoli BL-21 (Amersham Pharmacia), and expression of GST-Fish orGST alone was induced in 500 ml cultures via isopropyl-1-thio- $beta$ -D-galactopyranoside.Induced cells were pelleted and lysed in 4 ml of B-Per solution(Pierce, Rockford, IL). The debris was pelleted by centrifugation,and 200 µl of supernatant (containing ~2 µg of GST-Fish or GSTprotein) was incubated with 10 µl of glutathione-Sepharose-4Bbeads (Amersham Pharmacia) and 5 µl of ³⁵S-labeled Sim in vitro translation mix for 2 hr at 4°C. The beadswere washed five times with BC100N buffer (Ambrosetti et al.,1997) and then boiled with 2 µl of SDS gel loading buffer and8 µl of H₂O. The supernatants were electrophoresed on a 10% SDS-polyacrylamidegel along with 1 µl of the in vitro translation mixture (20% ofthe input used in the binding assays). The gel was dried and analyzedviaautoradiography.

To test Fish dimerization, 1-4 µg of purified GST-Fish was incubated with glutathione-Sepharose-4B beads in NETN (20 mM Tris-HCl,pH 8.0, 100 mM NaCl, 1 mM EDTA, and 0.5% NP40) at 4°C for 2 hr.This was followed by several washes with NETN. ³⁵S-labeled Fish protein was generated via an in vitro transcription/translationreaction (Promega) using fish cDNA clone 2-5 as template. Fivemicroliters of ³⁵S-labeled Fish were separately incubated with glutathione-Sepharose-4Bbeads in NETN at 4°C for 2 hr. The supernatant containing ³⁵S-labeled Fish was then incubated for 2 hr at 4°C with the GST-Sepharose-4Bbeads, which had been preincubated with GST-Fish. The beads werewashed several times with NETN, and bound protein was eluted withbuffer containing reduced glutathione (Amersham Pharmacia). Thesesamples, along with 2 µl of the in vitro translation mixture (40%of the input used in the binding assays), were mixed with SDSsample buffer, boiled, and electrophoresed on an 8% SDS-polyacrylamidegel. The gel was fixed in methanol/acetic acid (1:1), dried, andanalyzed viaautoradiography.

Schneider line 2 cell transient expression assays. Drosophila Schneider line 2 (S2) cells were cotransfected with the P[1.0slit-lacZ]reporter plasmid or the lacZ control vector C4PLZ along with combinationsof plasmids that provide a source of Sim, Tgo, Fish, and Dfr proteins.The reporter plasmid contained the slit 1 kb midline glial enhancerfragment cloned into the C4PLZ enhancer/tester vector (Whartonand Crews, 1993). Expression plasmids pAct-sim, pAct-tgo, pAct-fish,and pAct-dfr were made by subcloning cDNA fragments containingthe complete coding regions into pAct5C (sim, tgo, dfr) or pAct5CSRS(fish), each containing the Drosophila actin5C promoter and poly(A)site (Han et al., 1989; Sonnenfeld et al., 1997; K. Burtis, personalcommunication). S2 cells were transiently transfected using Ca₂PO4(Fehon et al., 1990). Transfections were performed in triplicateor more using 5 µg/plasmid and were normalized using 2.5 µg ofcopia-luc, which has a luciferase (luc) reporter (pGL3-Basic;Promega) under the control of the copia long terminal repeat (LTR)promoter. The cells were lysed 48 hr after transfection, and $beta$ -Galand luciferase assays were performed using a LacZ/ $beta$ -Gal QuantitationKit (Molecular Probes, Eugene, OR) and Luciferase Assay System(Promega),respectively.

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
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sim, fish, and dfr are expressed together in developing CNS midline cells

To address whether the sim, fish, and dfr genes might functionally interact to regulate development of the embryonic CNS midline,we first analyzed whether they exhibit overlapping expressionin developing midline cells. This was accomplished using anti-Fishand anti-Dfr sera, as well as a P[3.7sim-lacZ] marker that mimicssim midline expression (Nambu et al., 1991; Kasai et al., 1998).P[3.7sim-lacZ] embryos were immunostained using anti- $beta$ -gal andeither anti-Fish or anti-Dfr sera. Prominent overlapping expressionwas detected between Sim and Fish in developing CNS midline cellsfrom stage 8 throughout the remainder of germ band extension.Overlap was also detected in a subset of prospective foregut cells.Similar overlapping expression was also detected between Sim andDfr. Midline coexpression of Fish and Dfr was detected by immunostainingwild-type embryos with anti-Fish and anti-Dfr sera. Both genesare expressed together in the CNS midline throughout germ bandextension. Examples of this overlapping expression in germ band-extendedembryos are presented in Figure 1. In germ band-retracted embryos,Fish exhibited overlapping expression with Sim and Dfr in themidline glia (data not shown). Fish and Dfr were also detectedtogether in lateral cells of the thoracic ganglia and a subsetof ventral epidermal cells (data not shown). Consistent with previousstudies (Ma et al., 1998), Fish protein was not detected in thetrachea, a prominent site of Dfr expression (Anderson et al.,1995; Certel et al., 1996). These analyses indicated that sim,fish, and dfr are coexpressed in developing CNS midline cells.The midline expression of these three genes also overlaps thatof the slit gene, which is a downstream target of Sim (Whartonand Crews, 1993; Wharton et al., 1994).

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Figure 1. Coexpression of Sim, Fish, and Dfr in embryonic CNS midline cells detected via double-label immunostaining of P[3.7sim-lacZ] (A, B) and wild-type (C) embryos and confocal microscopy. A, A stage 9 P[3.7sim-lacZ] embryo immunostained with anti- $beta$ -gal (red) and anti-Fish (green) sera. Note strong overlapping expression (yellow) in the CNS midline cells. Fish is also strongly expressed in the lateral and cephalic neuroectoderm. B, A stage 10 P[3.7sim-lacZ] embryo immunostained with anti- $beta$ -gal (red) and anti-Dfr (green) sera. Note strong overlapping expression (yellow) in the CNS midline cells. Dfr is also strongly expressed in developing tracheal cells. C, A wild-type stage 11 embryo immunostained with anti-Fish (red) and anti-Dfr (green) sera. Note overlapping expression (yellow) in the CNS midline cells. Fish expression is not detected in tracheal cells. All views are ventral with anterior to left.

Genetic interactions reveal cooperative functions between sim, fish, and dfr

Both loss-of-function and gain-of-function assays were used to detect genetic interactions between sim, fish, and dfr. Significantly,a previous study had revealed genetic interactions between fish(also called Dichaete) and dfr (also called ventral veins lacking)mutants in CNS midline differentiation and Slit protein expression(Sánchez Soriano and Russell, 1998). We have extended these studiesto analyze potential cooperative interactions between sim, fish,and dfr in regulating slit gene transcription through use of aP[1.0slit-lacZ] marker. This reporter contains a portion of aslit intron that drives lacZ expression mimicking that of thenative slit gene in developing midline glia; P[1.0slit-lacZ] expressionis first detected in germ band-extended stage 11 embryos and ismaintained throughout the remainder of embryogenesis (Fig. 2A)(Nambu et al., 1991; Wharton and Crews, 1993; Wharton et al.,1994). fish null mutant embryos exhibited a misplacement and lossof midline glia, as detected via anti- $beta$ -gal immunostaining (Fig.2B). P[1.0slit-lacZ] was expressed normally in stage 11 fish mutantembryos, but during germ band retraction the number of midlineglia became reduced from wild type, and many cells were locatedat aberrant ventral positions within the nerve cord. Similar,although less severe, defects were observed in dfr mutant embryos,where some midline glia were displaced from their normal positions(Fig. 2C). Notably, $beta$ -gal-expressing midline glia were still detectedin both fish and dfr mutants, indicating that unlike Sim, Fishand Dfr are not absolutely required for P[1.0slit-lacZ] expressionor midline glial development.

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Figure 2. Genetic interactions between fish and dfr in CNS midline gene expression and development. Anti- $beta$ -gal immunostaining of stage 15 wild-type (A), fish⁸⁷ (B), dfr^E82 (C), and dfr^E82-fish⁸⁷ double mutant (D) embryos carrying the P[1.0slit-lacZ] marker. In addition, anti- $beta$ -gal immunostaining was also performed on stage 15 wild-type (E) and dfr^E82-fish⁸⁷ double mutant (F) embryos carrying the P[3.7sim-lacZ] marker. A, Note the predominantly dorsal positions of P[1.0slit-lacZ]-expressing midline glia in each segment of the ventral nerve cord in a wild-type embryo. B, In fish⁸⁷ mutant embryos there is a loss and disorganization of P[1.0slit-lacZ]-expressing midline cells. C, In dfr^E82 mutant embryos there is only modest misplacement of P[1.0slit-lacZ]-expressing midline cells. D, In dfr^E82-fish⁸⁷ double mutant embryos there is a dramatic loss of P[1.0slit-lacZ]-expressing cells. This phenotype is much more severe than that seen in either fish⁸⁷ (B) or dfr^E82 (C) single mutant embryos. E, In wild-type embryos the CNS midline cells express sim and are organized into segmentally reiterated clusters of cells along the ventral nerve cord. F, In dfr^E82-fish⁸⁷ double mutant embryos there is a severe decrease in sim expression and disorganization of midline cells. All views are sagittal with anterior to left.

We then used a dfr-fish double mutant strain to examine whether fish and dfr might act together to regulate midline gene expression.Embryos mutant for both fish and dfr were shown to exhibit muchmore severe defects in P[1.0slit-lacZ] expression than eitherfish or dfr single mutants. Although P[1.0slit-lacZ] was activatednormally in stage 11 dfr-fish double mutant embryos, there wasa striking loss of midline P[1.0slit-lacZ] expression during germband retraction (Fig. 2D). This synergistic effect strongly suggeststhat Fish and Dfr function together to regulate slit transcription.These functions may be mediated directly through Fish and Dfrbinding sites present in the slit 1 kb regulatory region (seebelow). Another, nonexclusive possibility is that Fish and Dfrmight indirectly control slit transcription by regulating theexpression of sim. To address this possibility we examined P[3.7sim-lacZ]expression in wild-type and dfr-fish embryos. Compared with wild-typeembryos, dfr-fish double mutants exhibited a severe decrease inP[3.7sim-lacZ] expression, a phenotype that first became apparentduring germ band retraction (Fig. 2E,F). Thus, fish and dfr alsoinfluence sim expression and hence may indirectly influence theexpression of a wide array of midlinegenes.

Because homozygous sim mutants exhibit severe CNS midline defects, it was not informative to analyze the phenotypes of fish-simor dfr-sim double mutants. Instead, we examined potential interactionsbetween fish and sim via a gain-of-function approach using theGal4/UAS targeted gene expression system (Brand and Perrimon,1993). A P[GMR-Gal4] strain that drives Gal4 expression in andbehind the morphogenetic furrow in the developing eye imaginaldisk was crossed to P[UAS-fish] and P[UAS-sim] strains. P[GMR-Gal4]/+;P[UAS-fish]/+animals exhibited a moderate eye roughening with disruption ofommatidia organization and loss of mechanosensory bristles (Mukherjeeet al., 2000) (Fig. 3A,D). In contrast, ectopic sim expressionresulted in essentially normal eye morphology (Fig. 3B,E). Theeffects of fish and sim coexpression revealed a nonadditive phenotype;there was a stronger disorganization of ommatidia and mechanosensorybristles than seen in flies expressing fish or sim alone, andthere was also a dramatic loss of eye pigmentation (Fig. 3C,F).These results indicated that ectopic expression of fish and simsynergistically alters normal eye development, and along withother data described below supports the hypothesis that thesegenes can interact functionally.

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Figure 3. Interactions between Fish and Sim detected via gain-of-function assay. Light microscope (A-C) or scanning electron microscope (D-F) analysis of eyes from adults in which ectopic Fish and/or Sim expression was driven in developing eye imaginal disks via P[GMR-Gal4]. A, D, A P[GMR-Gal4]/+; P[UAS-fish]/+ animal. Note that the eye is roughened, and there is a disorganization of ommatidia and loss of most mechanosensory bristles. There is a slight loss of eye pigmentation. B, E, A P[GMR-Gal4]/+; P[UAS-sim]/+ animal. Note essentially normal organization of ommatidia and mechanosensory bristles and uniform eye pigmentation. C, F, A P[GMR-Gal4]/+; P[UAS-sim]/P[UAS-fish] animal. Note more severe disorganization of ommatidia and mechanosensory bristles as well as a strong loss of eye pigmentation. A-C, Light microscope images at 20× magnification. D-F, Scanning electron microscope images at 1000× magnification.

Sim, Fish, and Dfr directly regulate slit transcription

Previous DNA sequence analysis of a 380 bp slit midline regulatory fragment indicated the presence of a single CME, throughwhich Sim:: Tgo heterodimers act (Wharton et al., 1994; Sonnenfeldet al., 1997). The CME is located within 300 bp from the distalend (farther from the promoter in the native slit gene) of thisfragment (Wharton et al., 1994). We additionally noted the presenceof an inverted TTCAAT repeat (TTCAATTTCATTGAA) located 20 bp proximalto the CME. This sequence resembles a (A/T)(A/T)CAAT consensusbinding site for Sox proteins, although to our knowledge, bindingof Sox proteins to a TTCAAT sequence has not been reported. Becausesequences present in an extended 1 kb slit DNA fragment are requiredfor normal levels of slit expression in vivo (Wharton and Crews,1993), we obtained additional DNA sequences. This analysis indicatedthat no other CMEs are present in the 1 kb slit DNA fragment.However, we did identify two perfect Dfr consensus binding sites(Certel et al., 1996), ATGCAAAT and CATAAAT, located within 500bp of DNA proximal to the CME (Fig. 4A). These two Dfr bindingsites are separated by ~150 bp and flank a consensus Fish bindingsite, TACAAT (Fig. 4A). These data suggest that Fish, Sim, andDfr may all bind to sites present in the 1 kb slit regulatoryDNA fragment. To test this possibility, DNA gel mobility shiftassays were performed using the Fish HMG domain and full-lengthDfr protein on double-stranded oligonucleotide probes correspondingto sequences from the slit 1 kb fragment. The Fish HMG domainbound strongly to a 26 mer probe containing the TACAAT site (Fig.4B). In contrast, Fish did not bind consistently to a 26 mer probecontaining both TTCAAT sites, suggesting that Fish can distinguishbetween closely related DNA sequences. Dfr protein bound verystrongly to a 33 mer probe that contained the ATGCAAAT site, andless strongly to a 32 mer probe containing the CATAAAT site (Fig.4B). Dfr bound the ATGCAAAT site both as an apparent monomer anda dimer, because two distinct bands with reduced mobilities weredetected. The 1 kb slit fragment thus may integrate the actionsof at least three different types of regulatory proteins, representedby Sim, Fish, and Dfr.

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Figure 4. The slit 1 kb midline regulatory region contains binding sites for Sim:: Tgo, Fish, and Dfr. A, Nucleotide sequence of a HinDIII/HinDIII restriction enzyme fragment from a slit gene intron (Wharton and Crews, 1993) that contains CNS midline regulatory elements. Indicated in bold are the single CME site through which Sim:: Tgo heterodimers act, two closely linked TTCAAT consensus Sox sites, a TACAAT Fish binding site, and ATGCAAAT and CATAAAT Dfr binding sites. Sequences corresponding to the double-stranded oligonucleotide probes used in gel mobility shift assays with the Fish HMG domain or Dfr protein are underlined. B, Gel mobility shift assays performed with purified Fish HMG domain or Dfr protein and sequences from the slit 1 kb regulatory region. Lane 1, Free TACAAT probe. Lane 2, TACAAT probe and Fish HMG domain protein. Note strong binding of Fish protein. Lane 3, Free TTCAAT probe. Lane 4, TTCAAT probe and Fish HMG domain protein. Note lack of detectable binding by Fish protein. Lane 5, Free ATGCAAAT probe. Lane 6, ATGCAAAT probe and Dfr protein. Note that Dfr binds strongly to this sequence as both an apparent monomer and a dimer (arrow). Lane 7, Free CATAAAT probe. Lane 8, CATAAAT probe and Dfr protein. Note that Dfr also binds to this sequence, although less strongly than to the ATGCAAAT sequence.

We next examined the ability of Fish, Dfr, Sim, and Tgo to directly control slit transcription using transient transcriptionassays in cultured Drosophila S2 cells (Fig. 5). The P[1.0slit-lacZ]construct was used as a reporter with various combinations ofplasmids that express Fish, Dfr, Sim, or Tgo. Fish modestly activatedP[1.0slit-lacZ] transcription (4 units of $beta$ -gal activity), indicatingthat in both yeast (Ma et al., 1998) and fly cells, Fish can functionas a direct transcriptional activator. Dfr resulted in littleif any activation of P[1.0slit-lacZ] (<1 unit), and Dfr and Fishtogether did not exhibit any increased activation over the levelsobserved for Fish alone. Neither Sim nor Tgo alone was able toactivate the P[1.0slit-lacZ] reporter, because only backgroundlevels of expression were detected (<0.4 units of activity). Furthermore,Sim and Tgo together yielded only minimal P[1.0slit-lacZ] activation(1 unit). These results imply that although Sim:: Tgo heterodimersstrongly activate expression of a P[6XCME-lacZ] reporter (>150units) that contains six multimerized CMEs (Sonnenfeld et al.,1997), additional factors are required to achieve high levelsof P[1.0slit-lacZ] expression. Significantly, the combinationof either Fish and Sim:: Tgo or Dfr and Sim:: Tgo both resultedin relatively high levels of P[1.0slit-lacZ] activation (23 unitsfor Fish and Sim:: Tgo and 12 units for Dfr and Sim:: Tgo). Thus,both Fish and Dfr strongly enhanced the ability of Sim:: Tgo heterodimersto activate slit transcription. Comparable levels of P[1.0slit-lacZ]activation (14 units) were observed when all four proteins wereexpressed together. Taken together, the DNA binding and transcriptionalactivation assays provide additional evidence that regulationof slit expression in the midline glia requires functional interactionsbetween Fish, Dfr, Sim, and Tgo.

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Figure 5. Fish and Dfr enhance Sim:: Tgo transcription of the P[1.0slit-lacZ] transgene in cultured Drosophila S2 cells. S2 cells were cotransfected with P[1.0slit-lacZ] reporter alone (1) or P[1.0slit-lacZ] with various combinations of the expression plasmids pAct-sim, pAct-tgo, pAct-fish, and pAct-dfr (2-10). Transfection efficiencies were normalized using a copia-luc plasmid. Cells were lysed 48 hr after transfection, and $beta$ -gal and luciferase activity were assayed. Normalized $beta$ -gal activity is expressed in arbitrary fluorescence units as the mean (SEM of 3-5 independent transfections). (1) 1.0slit-lacZ; (2) 1.0slit-lacZ + Fish; (3) 1.0slit-lacZ + Tgo; (4) 1.0slit-lacZ + Sim; (5) 1.0slit-lacZ + Dfr; (6) 1.0slit-lacZ + Fish + Dfr; (7) 1.0slit-lacZ + Sim + Tgo; (8) 1.0slit-lacZ + Sim + Tgo + Fish; (9) 1.0slit-lacZ + Sim + Tgo + Dfr; (10) 1.0slit-lacZ + Sim + Tgo + Fish + Dfr.

Interactions between Sim, Fish, and Dfr proteins

The ability of Sim, Fish, and Dfr to regulate P[1.0slit-lacZ] expression and the location of their respective DNA bindingsites in the 1 kb slit DNA fragment suggests that their regulatoryfunctions may involve direct protein-protein interactions. Weinitially addressed this possibility using yeast 2-hybrid assays,in which combinations of bait (fusions to the LexA-DNA bindingdomain) and prey (fusions to the B42 activation domain) constructsthat express full-length or truncated Sim, Fish, and Dfr proteinswere tested for their ability to activate expression of a LEU2reporter gene. Full-length Fish yielded strong interaction withboth full-length Sim and full-length Dfr (Fig. 6A). In addition,Fish exhibited the ability to self-associate, suggesting thatit may form homodimers. We then analyzed which regions of Simand Dfr associate with Fish. Interactions were detected betweenfull-length Fish and Sim bHLH-PAS and PAS constructs, but nota Sim bHLH-only construct (Fig. 6A). Thus, Fish specifically interactswith the PAS domain of Sim. Only a single PAS region was requiredfor this interaction, because Fish also exhibited interactionswith a Sim bHLH-PAS-A construct. Full-length Fish was also foundto interact with the POU domain of Dfr (Fig. 6A). This is consistentwith the ability of the vertebrate Sox2 protein to associate withthe POU domain of Oct3 (Ambrosetti et al., 1997). In an attemptto map which region of Fish is responsible for interactions withSim and Dfr, we used several bait constructs that express truncatedversions of Fish, including the HMG domain, NH₂-terminal region,COOH-terminal region, NH₂+HMG, HMG+COOH, or NH₂+COOH regions.None of these constructs exhibited consistent interaction withany Sim or Dfr prey construct. Although it is possible that structuraldeterminants present only on full-length Fish are required forinteractions with PAS or POU domains in the yeast 2-hybrid assay,on the basis of previous studies on Sox2 (Ambrosetti et al., 1997)it is likely that the Fish HMG domain is a key contributor tothese interactions.

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Figure 6. Fish directly associates with POU and PAS domain proteins. A, Interactions between Fish, Sim, and Drifter revealed via yeast 2-hybrid assays. The following combinations of bait and prey constructs were transformed into yeast and assayed for growth on Leu^- medium: (1) Fish/TrhbHLH-PAS; (2) Fish/PerL; (3) Fish/Per; (4) Fish/Sim; (5) Fish/SimPAS; (6) Fish/SimbHLH; (7) Fish/SimbHLH-PAS; (8) Fish/SimbHLH-PASA; (9) Fish/Fish; (10) Fish/Drifter; (11) Fish/DrifterPOU; (12) Fish/Pdm-1; (13) Fish/Pdm-2; (14) Fish/Oct-3; (15) Drifter/Sim; (16) Drifter/SimbHLH-PAS; (17) DrifterPOU/Sim; (18) DrifterPOU/SimbHLH-PAS. Note that interactions were detected between Fish and the POU domain of Drifter, as well as the PAS domain but not the bHLH region of Sim. No interactions were detected between any Sim and Drifter constructs. B, Binding of GST-Fish fusion protein to ³⁵S-labeled Sim generated via in vitro translation. Lane 1, In vitro-translated Sim analyzed via SDS-PAGE and autoradiography. Note a radiolabeled band at 73 kDa corresponding to full-length Sim protein, as well as a second band of lower molecular weight. Lane 2, In vitro-translated Sim does not bind GST. Sim protein was incubated with GST and glutathione-Sepharose resin. The mixture was washed, and the bound material was eluted and analyzed via SDS-PAGE and autoradiography. Note the absence of labeled Sim protein. Lane 3, In vitro-translated Sim binds to GST-Fish. Sim protein was incubated with GST-Fish and glutathione-Sepharose resin. The mixture was washed, and the bound material was eluted and analyzed via SDS-PAGE and autoradiography. Note the presence of labeled Sim proteins. C, Binding of GST-Fish fusion protein to ³⁵S-labeled Fish generated via in vitro translation. Lane 1, In vitro-translated Fish analyzed via SDS-PAGE and autoradiography. Note a major radiolabeled band at ~45 kDa corresponding to full-length Fish. Lane 2, In vitro-translated Fish does not bind efficiently to GST. Fish protein was incubated with GST and glutathione-Sepharose resin. The mixture was washed, and the bound material was eluted and analyzed via SDS-PAGE and autoradiography. Note the absence of labeled Fish protein. Lane 3, In vitro-translated Fish does bind GST-Fish. Fish protein was incubated with GST-Fish and glutathione-Sepharose resin. The mixture was washed, and the bound material was eluted and analyzed via SDS-PAGE and autoradiography. Note the presence of labeled Fish protein.

To verify the interactions between Fish and Sim and the self-association of Fish, we additionally performed GST pulldown assays.Fish and Sim interaction was tested using bacterially expressedGST or GST-Fish fusion protein, and ³⁵S-labeled Sim generated via in vitro translation. The ³⁵S-labeled Sim migrated on an SDS polyacrylamide gel as a doublet,with one band near the predicted molecular weight of Sim protein(73 kDa) and the second at a somewhat lower apparent molecularweight (Fig. 6B). Equal amounts of labeled Sim protein were incubatedwith either GST or GST-Fish, and the mixtures were subjected toglutathione-Sepharose chromatography followed by SDS-PAGE andautoradiography. As expected, Sim did not bind to the GST becauseno labeled bands were detected (Fig. 6B). However, Sim did associatewith GST-Fish, because both of the labeled Sim bands were observed(Fig. 6B). These data confirm the results of the yeast 2-hybridassays and indicate that Fish and Sim are capable of direct physicalassociation. Similar GST pulldown assays were performed to verifyFish self-association using GST-Fish and ³⁵S-labeled in vitro-translated Fish protein. The major band presentin the ³⁵S-labeled Fish reaction migrated at ~45 kDa (Fig. 6C), close tothe predicted molecular weight of Fish protein (40 kDa). This45 kDa band was specifically bound by GST-Fish but not GST alone(Fig. 6C). This result also confirmed the yeast 2-hybrid dataindicating that Fish is able to self-associate.

No interactions were detected between Sim bait and Dfr prey constructs in the yeast 2-hybrid assays (Fig. 6A), indicatingthat at least in yeast, they do not associate directly. Becauseboth proteins did associate with Fish, we tested whether Fishmight facilitate interactions between Sim and Dfr. This was pursuedusing Sim bait, Dfr prey, and a pDB20-fish construct to expressfull-length native Fish in yeast (see Materials and Methods).The combinations of pDB20-fish and either Sim bait or Dfr preydid not result in any detectable interaction, as indicated bythe inability of transformed yeast cells to activate LEU2 reportergene expression and grow on leu medium (Fig. 7). However, the simultaneous presence of pDB20-fish,Sim bait, and Dfr prey constructs did permit growth on leu medium (Fig. 7), indicating that Sim, Fish, and Dfr are ableto form a ternary complex in yeast cells.

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Figure 7. Fish, Sim, and Dfr can form a functional ternary complex in yeast cells. Combinations of full-length Sim bait, full-length Dfr prey, and full-length Fish expression constructs were tested for their abilities to interact in yeast cells. A, A combination of Sim bait and native Fish did not activate LEU2 expression, as indicated by the absence of cell growth on medium lacking leucine. B, A combination of Dfr prey and native Fish did not activate LEU2 expression, as indicated by the absence of cell growth on medium lacking leucine. C, A combination Sim bait, Dfr prey, and Fish did result in activation of LEU2 expression, as indicated by significant cell growth on medium lacking leucine. Fish can facilitate interactions between Sim bait and Dfr prey in yeast cells.

Additional yeast 2-hybrid assays were performed to examine potential interactions between Fish and other PAS and POU proteins.Full-length Fish interacted with the POU domains of both DrosophilaPdm-1 and Pdm-2, which are involved in embryonic segmentationand nervous system development (Bhat et al., 1995; Yeo et al.,1995; Ma et al., 1998), as well as full-length mouse Oct3 (Fig.6A). Fish also interacted with the bHLH-PAS region of DrosophilaTrachealess (Trh), a protein required for formation of severaltypes of tubular tissues (Wilk et al., 1996). As well, Fish interactedwith a PAS domain-containing fragment of Drosophila Per (Per-C2)(Huang et al., 1995), a PAS-only protein that associates withthe Timeless protein and plays a key role in regulating biologicalrhythms (for review, see Hardin, 1998; Young, 1998). Because Fishalso interacted with PerL, a mutant version of Per that exhibitsreduced ability to bind Timeless (Gekakis et al., 1995), it appearsthat distinct residues are important for Per/Fish versus Per/Timelessinteractions. Together, these data indicate that Fish can associatewith multiple POU and PAS domain proteins and suggest that functionalinteractions between Sox, PAS, and POU proteins may be importantin diverse developmental and physiologicalprocesses.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Functions of Sim, Fish, and Dfr in the regulation of CNS midline gene expression

The Drosophila slit gene encodes a large extracellular protein that is required for normal midline glial migration and axonprojection patterns (Rothberg et al., 1988, 1990). slit expressionin the CNS midline glia was mimicked by a P[1.0slit-lacZ] transgenethat is first expressed in fully germ band-extended embryos (Whartonand Crews, 1993). This expression is completely dependent on thefunctions of the bHLH-PAS protein Sim, because sim mutant embryosexhibit a complete absence of P[1.0slit-lacZ] expression (Nambuet al., 1991). In this study, we show that the combined functionsof the Sox protein Fish and the POU domain protein Dfr are alsoessential for P[1.0slit-lacZ] expression, because dfr-fish doublemutant embryos exhibit a dramatic loss of P[1.0slit-lacZ] expressionin germ band-retracted embryos. Additionally, Fish and Dfr significantlyenhanced the ability of Sim and Tgo to activate P[1.0slit-lacZ]expression in cultured Drosophila S2cells.

The 1 kb slit midline regulatory region was found to contain binding sites for Fish and Dfr, as well as a single CME throughwhich Sim:: Tgo heterodimers function. Fish bound strongly toa TACAAT site and Dfr bound to two sites, ATGCAAAT and CATAAAT,that flank the Fish site within a 150 bp interval. Removal ofthe Fish and Dfr binding sites reduces slit expression, becausea P[380slit-lacZ] strain that contains the CME but not the Fishor Dfr binding sites exhibits decreased levels of embryonic midlineexpression compared with P[1.0slit-lacZ] (Wharton and Crews, 1993).Fish did not consistently bind to two TTCAAT sequences locatedclose to the CME; however, given the proximity of these sites,it will be of interest to determine whether Fish and Sim:: Tgomight bind these sequences cooperatively. We also determined thatFish protein directly associates with the PAS domain of Sim andthe POU domain of Dfr. In addition, all three proteins were ableto form a ternary transcriptional regulatory complex in yeast.Together, these results provide strong evidence that these proteinsact together to directly regulate midline gene expression. Onemodel for the functions of these proteins is that although Sim::Tgo heterodimers are sufficient to activate embryonic expressionof P[1.0slit-lacZ], Fish and Dfr are required to maintain highlevels of LacZ expression (Fig. 8).

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Figure 8. A model for regulation of P[1.0slit-lacZ] expression in the CNS midline via interactions between Sim, Tgo, Fish, and Dfr. In wild-type embryos (A) the binding of a Sim:: Tgo heterodimer to the CME and Fish and Dfr to nearby sites results in the formation of a ternary regulatory complex that permits sustained midline P[1.0slit-lacZ] expression. In the absence of Sim (B), Fish and Dfr are not sufficient to activate expression of P[1.0slit-lacZ]. In the absence of both Fish and Dfr (C), the initial presence of Sim is sufficient to activate midline P[1.0slit-lacZ] expression; however, this expression is not maintained in germ band-retracted dfr-fish mutant embryos. D, Drifter; F, Fish; S, Sim; T, Tgo. Dots indicate direct protein-protein interactions.

Functional interactions between Sim, Fish, and Dfr may also regulate the midline expression of other genes, including simand breathless (btl). Thus, sim has autoregulatory functions (Nambuet al., 1991), and we have shown that the combined functions ofdfr and fish are also required for sustained midline sim expression.In addition, a 2.8 kb interval in the P[3.7sim-lacZ] transgeneused in this study contains six evolutionarily conserved CMEs(Kasai et al., 1998) as well as several consensus Fish and Dfrbinding sites. btl encodes an FGF receptor homolog whose expressionin the CNS midline and tracheal cells has been shown to depend,respectively, on Dfr as well as Sim and Tgo, or Trh and Tgo (Andersonet al., 1996; Ohshiro and Saigo, 1997). A 200 bp btl midline/trachealregulatory region contains three evolutionarily conserved CMEs(Ohshiro and Saigo, 1997). Inspection of this region also revealedthe presence of a conserved consensus ATCAAT Fish binding sitelocated in a 40 bp interval between CME2 and CME3, as well asa conserved consensus GATAAAT Dfr binding site (Anderson et al.,1996) located 40 bp downstream of CME3. Thus, functional interactionsbetween Sim, Fish, and Dfr could be a general mechanism to regulategene transcription during CNS midlinedevelopment.

Like other Sox proteins, Fish can influence transcription through DNA bending, direct transcriptional activation, and protein-proteininteractions. It will be of interest to determine the relativecontributions of these activities in regulating slit expression.In this regard, Sox proteins may act in distinct capacities dependingon the presence of other regulatory proteins and the organizationof control elements in a specific target gene. For example, closerange interactions between Sox2 and Oct3 are required to synergisticallyactivate a distal enhancer element from the vertebrate fgf4 gene(Yuan et al., 1995; Ambrosetti et al., 1997). Increasing the distancebetween the Sox2 and Oct3 binding sites from 3 to 6 bp abolishesthe ability of these proteins to activate transcription (Ambrosettiet al., 1997). In contrast, Sox2 represses Oct4-induced activationof a preimplantation enhancer from the mouse osteopontin geneby acting at a site 39 bp away from the Oct4 binding site (Botquinet al., 1998). This is similar to the interactions between Fishand Dfr through nonadjacent binding sites in the slit 1 kb midlineenhancer. These findings indicate that there are different mechanismsthrough which Sox and POU domain proteins can interact to regulatetranscriptional processes. Significantly, in the native fgf4,osteopontin, and slit genes, the relevant regulatory regions areall located several kilobases downstream of the promoter. Thissuggests that in addition to local DNA bending activities, thein vivo functions of Sox proteins may also involve DNA loopingevents (Lamb and Rizzino, 1998). Because Sry and presumably otherSox proteins bind DNA as a monomer (Werner et al., 1995), DNAlooping could be mediated via Sox protein dimerization, as detectedfor Fish and LSox5 and Sox6 proteins (Lefebvre and de Crombrugghe,1998), as well as through association between Sox and PAS or POUdomainproteins.

Conserved PAS, Sox, and POU regulatory interactions in nervous system development?

There are several examples of functional association between vertebrate HMG domain and POU domain proteins (Zwilling et al.,1995; Ambrosetti et al., 1997; Botquin et al., 1998; Kuhlbrodtet al., 1998), and our studies have revealed similar associationbetween Drosophila Sox and POU proteins. In addition, we haveidentified novel interactions between Sox and PAS domain proteins.Given the considerable sequence divergence between the PAS domainsof Sim or Trh and Per, the ability of Fish to directly associatewith each of these proteins suggests that interactions betweenSox and PAS domain proteins may also be widespread. In this regardwe have found that the mouse Sox2 protein, which contains an HMGdomain highly related to that of Fish, also associates with Simand Per (Y. Gao and J. R. Nambu, unpublished results). In addition,midline-targeted expression of Sox2 has been shown to partiallyrescue the axon scaffold defects in fish mutant embryos (SánchezSoriano and Russell, 1998). Although the precise mechanism ofPAS/Sox association is not clear, our results indicate that asingle PAS region is sufficient for binding to a Sox protein,and they suggest that the HMG domain is crucial for this interaction.Further analyses of the regulatory interactions between Sim, Fish,and Dfr may ultimately provide a useful paradigm for a betterunderstanding of the widespread functions of PAS, Sox, and POUgenes in vertebrate neural development, and their involvementin specific human congenital disorders that result in deafness,obesity, and mental retardation (Pevny and Lovell-Badge, 1997;Crews, 1998; Crews and Fan, 1999; Latchman, 1999; McEvilly andRosenfeld, 1999; Wegner, 1999).

  FOOTNOTES

Received Sept. 23, 1999; revised March 23, 2000; accepted March 27, 2000.

This work was supported by grants from the March of Dimes and National Institutes of Health (NIH) to J.R.N., NIH Grant NS28743to W.A.J., and grants from the National Institute of Child Healthand Human Development and National Science Foundation to S.T.C.K.C. was supported by an NIH Genetics Training Grant. We are indebtedto Lisa Dailey for providing us with Sox2 and Oct3 cDNA clones,Steve Poole for providing us with pdm-1 and pdm-2 cDNA clones,and Michael Rosbash for providing period yeast 2-hybrid constructs.In addition, we gratefully acknowledge Merrill Shaffer, XiaoliangShan, and Kahlin Clark for assistance in generating yeast 2-hybridconstructs.
Correspondence should be addressed to Dr. John R. Nambu, Biology Department, Morrill Science Center, University of Massachusetts,Amherst, MA 01003. E-mail: jnambu{at}bio.umass.edu.

E. Niemitz's present address: Predoctoral Training Program in Human Genetics, Johns Hopkins University School of Medicine,Baltimore, MD21205.

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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