DLG-1 Is a MAGUK Similar to SAP97 and Is Required for Adherens Junction Formation

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Vol. 12, Issue 11, 3465-3475, November 2001

DLG-1 Is a MAGUK Similar to SAP97 and Is Required for Adherens Junction Formation

Bonnie L. Firestein,^* and Christopher Rongo ^§

^*Department of Cell Biology and Neuroscience and The Waksman Institute, Department of Genetics, Rutgers University, Piscataway, NJ 08854

Submitted May 22, 2001; Revised August 17, 2001; Accepted August 23, 2001
Monitoring Editor: Mary C. Beckerle

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cellular junctions are critical for intercellular communication and for the assembly of cells into tissues. Cell junctionsoften consist of tight junctions, which form a permeability barrierand prevent the diffusion of lipids and proteins between cellcompartments, and adherens junctions, which control the adhesionof cells and link cortical actin filaments to attachment siteson the plasma membrane. Proper tight junction formation and cellpolarity require the function of membrane-associated guanylatekinases (MAGUKs) that contain the PDZ protein-protein interactiondomain. In contrast, less is known about how adherens junctionsare assembled. Here we describe how the PDZ-containing proteinDLG-1 is required for the proper formation and function of adherensjunctions in Caenorhabditis elegans. DLG-1 is a MAGUK proteinthat is most similar in sequence to mammalian SAP97, which isfound at both synapses of the CNS, as well as at cell junctionsof epithelia. DLG-1 is localized to adherens junctions, and DLG-1localization is mediated by an amino-terminal domain shared withSAP97 but not found in other MAGUK family members. DLG-1 recruitsother proteins and signaling molecules to adherens junctions,while embryos that lack DLG-1 fail to recruit the proteins AJM-1and CPI-1 to adherens junctions. DLG-1 is required for the properorganization of the actin cytoskeleton and for the morphologicalelongation of embryos. In contrast to other proteins that havebeen observed to affect adherens junction assembly and function,DLG-1 is not required to maintain cell polarity. Our results suggesta new function for MAGUK proteins distinct from their role incellpolarity.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell adhesion facilitates the assembly of individual cells into organized tissues, and several different cell adhesion mechanismsfulfill this role (Gumbiner, 1996). One of these adhesion mechanismsis the formation of the tight junction or zonula occludens, whichfunctions to regulate the permeability of the cell layer and topolarize the cell surface into apical and basolateral compartments(Mitic and Anderson, 1998). Tight junctions (in vertebrates) andseptate junctions (in invertebrates) maintain the separation betweenthe apical and basolateral surfaces by hindering the diffusionof lipids and proteins (Powell, 1981; van Meer et al., 1986; vanMeer and Simons, 1986; Gumbiner, 1987). In contrast to tight junctions,a second mechanism of cell adhesion is the adherens junction,which is responsible for maintaining adhesion between neighboringcells and is important for intercellular communication (Muller,2000; Vasioukhin and Fuchs, 2001).

While many proteins have important roles in assembling these junctions, mutations in these proteins result in large defectsin cell polarity as well. For example, mutations in the Drosophilagenes bazooka (baz), crumbs (crb), discs lost (dlt), scribble(scrib), lethal (1) discs large (dlg), and lethal giant larvae(lgl), and the Caenorhabditis elegans gene let-413 disrupt epithelialcell polarity and prevent the formation of cell junctions (Legouiset al., 2000; Muller, 2000). Because of the large-scale defectsin cell polarity caused by mutations in these genes, it is notclear whether they have a direct role in junction formation orif the failure to form junctions in mutants is due to generaldefects in cellpolarity.

BAZ, DLG, SCRIB, LET-413, and DLT each contain one or more PDZ domains, which are stretches of approximately 90 amino acidsthat bind to a consensus sequence at the extreme carboxyl terminiof other proteins (Doyle et al., 1996; Songyang et al., 1997).PDZ-containing proteins play a dual role in establishing polarityand assembling cell surface signaling molecules into protein complexesin a number of cell types and species, demonstrating the generalimportance of these proteins. For example, the C. elegans PDZproteins LIN-2, LIN-7, and LIN-10 are thought to form a complexthat is involved in mediating basolateral membrane localizationof the LET-23 EGF receptor in vulval epithelial cells (Kaech etal., 1998; Rongo et al., 1998; Whitfield et al., 1999). In mammals,members of the membrane-associated guanylate kinase (MAGUK) family,which contain 3 PDZ domains, play an integral role in targetingglutamate receptors and effector molecules to excitatory synapses(Kim et al., 1995; Kornau et al., 1995; Brenman et al., 1996;Kim et al., 1996; Kornau et al., 1997). A better understandingof the functional role of PDZ proteins might elucidate universalmechanisms for cell polarity and the formation of celljunctions.

Bossinger and colleagues have recently shown that gene finder prediction C25F6.2 is similar in sequence to MAGUK family members,and they have named the sequence dlg-1 (Bossinger et al., 2001).Nematodes knocked down for dlg-1 function by RNAi fail to formproper adherens junctions and arrest as twofold stage embryos.To better understand the formation of adherens junction, we havecloned DLG-1 and show here that this C. elegans protein contains3 PDZ domains, an SH3 domain, and a yeast guanylate kinase homologydomain, most similar to the SAP97 MAGUK family member found atcell junctions and synapses in mammals (Muller et al., 1995).We find that this protein localizes to adherens junctions of theepidermis, intestine, and pharynx of embryos and adult nematodes,and that the first 186 amino acids are sufficient for this localization.Embryos deficient in DLG-1 show abnormal adherens junction formationat the ultrastructural level, and they fail to localize the adherensjunction proteins AJM-1 and CPI-1 to cell junctions. Furthermore,the actin cytoskeleton in dlg-1(RNAi) embryos is disorganized,suggesting that like the cadherin-catenin system, DLG-1, alsoplays a role in coordinating the actin network with adherensjunctions.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Strains

The following strains were used: let-413(s128), hmp-1(zu278), hmp-2(zu364), zuEx24[hmp-1::gfp], hmr-1(zu389), mcEx[let-413::gfp],jcIs1[ajm-1::gfp].

DLG-1 cDNA

Based on Kohara expressed sequence tags, we sequenced several dlg-1 cDNA clones (a kind gift from Y. Kohara, National Instituteof Genetics, Mishima, Japan), including yk333g2, yk435h12, yk481e2,yk348h11, and yk481c12. To identify the 5' end of dlg-1, we isolatedtotal RNA by homogenizing mixed stage N2 nematodes in 200 mM LiCl,20 mM EDTA, 20 mM Tris Cl pH 7.8, and 2% SDS. The RNA was extractedseveral times with phenol and precipitated with ethanol. RT-PCRwas conducted by reverse transcribing 5 µg total RNA with theuse of AMV reverse transcriptase and oligo dT₁₅ as a primer (Promega,Madison, WI). A single 1.2-kb PCR product was amplified from thecDNA pool with the use of a primer for the SL1 leader (5'-GGTTTAATTACCCAAGTTTGAG-3')and a primer unique to dlg-1 (5'-GACCCGCCAAAGTTTCCTCCAATTGG-3'),cloned into pBluescript (Stratagene, LaJolla, CA), and sequenced.The cDNA sequence has been submitted to GenBank (Accession numberAF406786)

DLG-1 Expression Constructs

The dlg-1::gfp transgenes were made by ligating an EcoRI/XhoI fragment from the cosmid C25F6 to sequences encoding GFP andthe unc-54 3'UTR (pPD95.75, from A. Fire, Carnegie Institute ofWashington, Baltimore, MD). Transgenic strains were isolated bymicroinjecting the resulting plasmid (50 ng/µl) with the use ofrol-6(su1006dm) (C. Mello, University of Massachusetts MedicalCenter, Worchester, MA) as a cotransformation marker. Mutant versionsof DLG-1::GFP were engineered using PCR. Three different lineswere analyzed for each construct; all three had similarlocalization.

Fluorescent Microscopy

Immunohistochemistry of embryos and larvae was performed as described (Finney and Ruvkun, 1990). Anti-PKC-3 antibodies (Y.Tabuse, NEC Fundamental Research Laboratories, Ibaraki, Japan)were used as described (Tabuse et al., 1998). Actin filamentswere visualized in embryos with rhodamine-phalloidin (MolecularProbes), as described (Costa et al., 1997). LET-413::GFP (M. Labouesse),AJM-1::GFP and HMP-1::GFP (J. Hardin), and DLG-1::GFP eggs andlarvae were mounted and visualized on 2% agarose pads. Fluorescentimages were observed with the use of a Zeiss (Oberkochen, Germany)Axioplan II and 63X1.4NA objective and captured with a SensiCam(Cooke, Auburn Hills, MI) with the use of ImagePro v4.1 (MediaCybernetics, Silver Spring, MD) and VayTek v6.2 software (VayTek,Inc., Fairfield, IA). Animals were optically sectioned (0.25 µm),and out-of-focus light was removed with a constrained interativedeconvolution algorithm(VayTek).

RNA-mediated Interference

A dlg-1 cDNA in pBluescript, yk333g2 (Y. Kohara), was used as a template to generate dlg-1 sense and antisense transcripts.For cpi-1 RNAi, a 300 bp exon was PCR amplified from genomic DNAcorresponding to sequence F38E11.3 and was ligated into pBluescriptso that sense and antisense transcripts could be synthesized.Annealed transcripts were injected into worms to induce RNAi (Fireet al., 1998). An XhoI fragment from the dlg-1 cDNA and the cpi-1PCR product were also ligated between two T7 promoters in thepPD129.36 vector (A. Fire), and the resulting plasmids (CR254and CR255, respectively) were introduced into HT115(DE3) Escherichiacoli. E. coli harboring CR254 or CR255 were fed to nematodes toinduce RNAi as described (Kamath et al., 2000; Timmons and Fire,1998). RNAi by injection and by feeding gave similar results;however, stronger phenotypic expressivity and penetrance wereobserved with the feeding method. RNAi data described in the textand figures reflects data from the feeding method. The empty pPD129.36vector was used as a negative control in feeding experiments,and the resulting worms are shown as wild-type controls in allfigures.

Electron Microscopy

Embryos were isolated from egg shells by digestion with chitinase (Sigma, St. Louis, MO) for 20 min in 120 mM NaCl, 40 mMKCl, 3 mM CaCl₂, 3 mM MgCl₂, and 5 mM HEPES pH7.2. Embryos werefixed in 4% paraformaldehyde/2% glutaraldehyde and postfixed in1% osmium tetroxide and uranyl acetate. Twofold stage embryoswere dehydrated, embedded in epon, and sectioned. Sections of50 nm were contrasted with uranyl acetate and observed for transmissionelectronmicroscopy.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

DLG-1 Is a PDZ Domain Protein that Is Localized to Adherens Junctions

The C. elegans genome contains ~50 genes predicted to contain at least 1 PDZ domain (Bargmann, 1998). Predicted gene C25F6.2encodes the sole protein similar to MAGUK proteins of the diskslarge family and therefore has been named dlg-1 for discs largelike protein (Bossinger et al., 2001). Genefinder algorithms oftenmake incorrect predictions of 5' and 3' sequences; thus, to determinethe correct protein sequence for dlg-1, we sequenced several dlg-1cDNA clones from the Y. Kohara library(Kohara, 1996). We alsoisolated and reverse transcribed RNA from mixed stage nematodes.The dlg-1 5'end was amplified by RT-PCR from cDNA with the useof primers specific for dlg-1 sequences and the SL1 transspliceleader sequence. Our sequencing results of the Kohara clones andRT-PCR products suggest that dlg-1 generates a single mRNA product.DLG-1 protein is predicted to encode 967 amino acids with aminoand carboxy-terminal sequences that differ from the original genefinderprediction that has been reported (Bossinger et al., 2001). DLG-1contains three PDZ domains, an SH3 domain, and a yeast guanylatekinase homology domain (Figure 1A), and is 38%, 38%, 28%, and34% identical to the MAGUK family members SAP97, SAP102, PSD-95,and Drosophila DLG, respectively (Woods and Bryant, 1991; Choet al., 1992; Kistner et al., 1993; Muller et al., 1995; Mulleret al., 1996). The amino terminal sequences of MAGUK proteinsare thought to contain important sequences for their subcellularlocalization and regulation, and these sequences often divergebetween family members. For example, the amino-terminus of PSD-95contains cysteine residues that allow the palmitoylation and thusmembrane association of this protein, the amino-terminus of SAP102binds to zinc, and although the SAP97 amino terminus is importantfor localization, it is not palmitoylated and does not bind tozinc (Craven et al., 1999; El-Husseini et al., 2000a,b; Firesteinet al., 2000; Wu et al., 1998a). Interestingly, the amino terminalsequence of DLG-1 is conserved (34% identity, 54% similarity)with the amino terminal 65 amino acids of SAP-97 (Figure 1B),a MAGUK protein found at mammalian synapses and epithelial celljunctions.

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Figure 1. DLG-1 is a MAGUK protein most similar to SAP97. (A) Deduced amino acid sequence of DLG-1 with PDZ domains in blue, SH3 domain in red, and guanylate kinase domain in gray. (B) Alignment of the amino-terminal 99 amino acids of DLG-1 with SAP97. Identical residues are indicated in black, whereas conserved residues are indicated in gray. (C) Schematic diagrams of the DLG-1:: GFP chimeric proteins. Embryos expressing DLG-1:: GFP (green) in intestine (D) and hypodermis (E) are shown with DAPI-stained nuclei (blue). Adult worms express DLG-1:: GFP in the Pnp epithelial cells (F) and lateral seam cells (G). Scale bar represents 10 µm.

The Conserved Amino-Terminus of DLG-1 Directs DLG-1 Localization to Adherens Junctions

Because many of the MAGUK proteins like SAP97 are found both in neurons and epithelial cells, we wanted to visualize whereDLG-1 was expressed and localized. Therefore, we constructed aGFP fusion gene by inserting GFP sequences at the carboxy terminusof DLG-1 (Figure 1C). Sequences for the resulting DLG-1::GFP chimericprotein were ligated to 5 kb of dlg-1 upstream promoter sequences.We introduced this construct into the C. elegans germline andfound that the resulting fusion protein is situated at adherensjunctions exclusively in epithelial cells of embryonic and adultepidermis, intestine, and pharynx (Figure 1D,E,F, n = 43/43).This pattern is also seen when embryos are stained with monoclonalantibodies that recognizes the mammalian PSD-95 (Figure 2, n =30/30). DLG-1::GFP is not expressed in neurons, and we did notdetect DLG-1 in the nervous system with the use of anti-PSD-95antibodies.

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Figure 2. DLG-1 is localized to adherens junctions and required for AJM-1:: GFP localization. Immunostaining of embryos that express AJM-1:: GFP (green, A, D, G, J, M) with anti-PSD-95 antibodies (red, B, E, H) or with anti-PKC-3 antibodies (red, K, N). Nuclei are stained with DAPI (blue). Merged images (C, F, I, L, O) contain a 10 µm scale bar. AJM-1:: GFP and DLG-1 colocalize to adherens junction on the epidermis (A-C, lima bean stage) and in the intestine (D-F, tadpole stage) of wild-type embryos. (G-I, twofold stage) AJM-1:: GFP is found in small punctate structures between cells in dlg-1(RNAi) embryos No DLG-1 protein is detected in these embryos. (J-L, gastrulating embryo) AJM-1:: GFP is found at intestinal adherens junctions (green) whereas PKC-3 is localized to the apical surface of these cells (red) in wild-type embryos. (M-O, gastrulating embryo) AJM-1:: GFP is found in punctate structures, but PKC-3 is found at the apical surface of cells from dlg-1(RNAi) embryos.

To identify the domain of DLG-1 that is responsible for its localization to adherens junctions, we generated mutant versionsof the DLG-1::GFP transgene that contained different domains ofthe DLG-1 protein (Figure 1C). The resulting transgenes were introducedinto the C. elegans germline and the resulting chimeric proteinsanalyzed for their subcellular localization. DLG-1(1-7)::GFP,which contains the first seven amino acids of DLG-1 fused to GFP,fails to be localized to adherens junctions and is entirely cytosolic(n = 54/54). In contrast, the first 186 amino acids of DLG-1 aresufficient to direct localization of GFP to adherens junctions(Figure 1C, n = 18/18). This region of DLG-1 is conserved withSAP97, and recent results suggest that the same domain of SAP97is important for cell junction localization when observed in coloncarcinoma cells immortalized in culture (Wu et al., 1998a). Ourresults show that the 3 PDZ domains, the SH3 domain, and the guanylatekinase domain are not required for DLG-1 localization. Instead,we find that the amino-terminal domain functions as an adherensjunction localization signal in vivo in epithelial cells of intacttissue.

DLG-1 Is Required for Adherens Junction Assembly but Is Not Essential for Polarized Protein Targeting

The pattern of DLG-1 expression highly resembles that of the adherens junction protein AJM-1, which encodes the MH27 antigenand was previously known as JAM-1 (Köppen et al., 2001; Mohleret al., 1998; Podbilewicz and White, 1994; Priess and Hirsh, 1986;Raich et al., 1999; Wood, 1988). Indeed, DLG-1 colocalizes withAJM-1::GFP as evidenced by immunostaining (Figure 2A-F, n = 18/18).Bossinger and colleagues tested the role of DLG-1 in adherensjunction formation by injecting nematodes with double-strandeddlg-1 RNA to induce RNAi(Bossinger et al., 2001; Fire et al.,1998). They observed that dlg-1(RNAi) embryos form an irregularjunction of AJM-1 around the apex of the cells and that, as morphogenesisproceeds, the junction begins to fragment. Their results suggestthat DLG-1 might be needed to maintain the integrity of adherensjunctions rather than for the initial formation of the junctions.Because dlg-1(RNAi) embryos still possess trace amounts of DLG-1protein, particularly in their intestine and pharynx, an alternativeexplanation is that the phenotype of these embryos representsonly a partial loss of dlg-1 function (Bossinger et al., 2001).

Although injection of double-stranded RNA can induce RNAi, recent studies have shown that RNAi induced by feeding nematodesbacteria that express double-stranded RNA for the gene of interestcan induce stronger and more penetrant phenotypes by removingmore gene product (Kamath et al., 2000). Thus, we examined therole of DLG-1 in adherens junction formation by removing DLG-1with the use of the feeding method of double-stranded RNAi. RNAiwith dlg-1 RNA abolishes DLG-1::GFP expression (n = 23/25, ourunpublished results) and fluorescence from anti-PSD-95 antibodystaining (Figure 2H) in all tissues examined (n = 42/44). AnyDLG-1 protein that might remain in dlg-1(RNAi) embryos is belowour limit of detection. We performed DLG-1 RNAi on nematodes thatexpress AJM-1::GFP and found that dlg-1(RNAi) embryos do not formjunctions of AJM-1 around the apex of cells even at the earliestdevelopmental stages at which AJM-1::GFP can be detected (Figure2G, n = 32/36, and our unpublished results). In most dlg-1(RNAi)animals, AJM-1::GFP is found in small punctate structures betweencells (Figure 2G, n = 32/36) rather than showing a continuousring of localization at cell boundaries as in wild-type embryos(Figure 2A,D, n = 22/22). Our results show that DLG-1 is neededfor the initial localization of AJM-1 to adherens junctions, notjust to maintain AJM-1 in continuous and unfragmented bands aroundthe cells as originally suggested (Bossinger et al., 2001).

One simple explanation for AJM-1 mislocalization is that dlg-1(RNAi) embryos are incapable of localizing all cell surfaceproteins. For example, the dlg-1(RNAi) phenotype is similar tothat found in let-413 mutants, which globally disrupt epithelialcell polarity (Legouis et al., 2000). Thus, we examined proteinlocalization in the dlg-1(RNAi) embryos. Remarkably, PKC-3, anatypical PKC required for embryonic development (Wu et al., 1998b),is localized apically in the mutant embryos (Figure 2N, n = 22/24),as it is in wild-type embryos (Figure 2K, n = 24/28). Similarly,LET-413::GFP is correctly localized to the basolateral surfacein dlg-1(RNAi) mutants (n = 30/31), as it is in wild-type embryos(n = 18/18, our unpublished results). These results demonstratethat at least two apical and basolateral proteins are properlylocalized in dlg-1(RNAi) embryos and suggest that DLG-1 playsa relatively specific role in adherens junction formation withoutdisrupting gross aspects of cellpolarity.

To determine whether there are ultrastructural changes to adherens junctions in dlg-1(RNAi) embryos, we examined the adherensjunctions of hypodermal and intestinal cells by transmission electronmicroscopy. In wild-type embryos, adherens junctions form electron-densestructures between membranes of adjacent cells near their apicalsurfaces (Figure 3A, n = 20/20). In dlg-1(RNAi) embryos, the electrondense junctions are often missing (Figure 3B, n = 22/26) or brokeninto discontinuous structures (Figure 3C, n = 4/26). Gaps oftenform between adjacent cells (n = 13/26), suggesting that the adhesiveproperties of the junctions are diminished.

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Figure 3. Abnormal ultrastructure of adherens junctions in dlg-1(RNAi) embryos. (A) Electron microscopy of an adherens junction (arrow) in a wild-type embryo. (B) Electron-dense adherens junction material is often missing in dlg-1(RNAi) embryos. Arrowheads point to gaps that have formed between adjacent membranes. (C) When adherens junctions are visible in dlg-1(RNAi) embryos, they are often discontinuous (arrowheads). Scale bar is 200 nm.

DLG-1 Is Required for Proper Elongation

To determine if DLG-1 is involved in the function of adherens junctions during embryogenesis, we analyzed dlg-1(RNAi) embryoswith the use of Nomarski interference microscopy. C. elegans embryosundergo two major morphogenetic movements during embryogenesisthat require adherens junctions: ventral enclosure and elongation(Sulston et al., 1983; Priess and Hirsh, 1986; Williams-Massonet al., 1997; Costa et al., 1998). During ventral enclosure, thefree edges of epidermis migrate to the ventral surface of theembryo, where they form new adherens junctions and thereby sealup the epithelial sheet (Williams-Masson et al., 1997). Mutationsthat prevent ventral closure fail to seal the ventral epitheliaand result in embryos that rupture at elongation (Raich et al.,1999). After ventral enclosure, actin filament bundles at adherensjunctions contract to change the shape of epithelial cells fromcircumferentially elongated to longitudinally elongated (Costaet al., 1997; Costa et al., 1998). These coordinated shape changesresult in the elongation of the nematode body along the anteroposterioraxis. Mutations that prevent elongation result in short embryoswith a bulged appearance (Williams and Waterston, 1994; Costaet al., 1998). We found that dlg-1(RNAi) embryos undergo ventralenclosure (Figure 4B, n = 38/38), as do wild-type embryos (Figure4A, n = 25/25), suggesting that DLG-1 is not required for thataspect of adherens junction function. However, unlike wild-typeembryos (Figure 4C, n = 29/29), dlg-1(RNAi) embryos fail to elongate(Figure 4D, n = 33/33). Taken together, these results suggestthat DLG-1 is not required for adherens junction-dependent filopodialpriming and cell movement during ventral enclosure but is necessaryinstead for cell shape changes required for elongation.

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Figure 4. DLG-1 is required for elongation and proper organization of actin filaments. (A-D) Nomarski interference microscopy of embryos. Wild-type (A) and dlg-1(RNAi) (B) embryos undergo proper ventral enclosure during gastrulation. However, unlike wild-type threefold embryos (C), dlg-1(RNAi) embryos fail to elongate and often contain large vacuoles (arrowhead). (E-I) Rhodamine-phalloidin staining of filamentous actin. Wild-type twofold embryos (E) develop an unelongated pharynx with radially-oriented actin filaments, which elongates into a complete pharynx (F) in threefold embryos. (G) The hypodermis of wild-type embryos contains circumferential filaments (cf) that wrap around the nematode, and adherens junction filaments (ajf) that have contracted circumferentially. The label "mf" indicates actin filaments of the longitudinal muscles. (H) In contrast, the pharynx of a dlg-1(RNAi) embryo fails to elongate and contains disorganized actin filaments. The labels "mc" and "tb" indicate metacorpus and terminal bulb, respectively. (I) The hypodermis of dlg-1(RNAi) embryos contains regions that lack circumferential actin bundles (black arrowhead). Adherens junction filaments are found at the adherens junctions of lateral hypodermis but have failed to contract circumferentially. Scale bar is 10 µm.

dlg-1(RNAi) Embryos Show Abnormal Actin Bundles

Because dlg-1(RNAi) embryos show a defect in elongation, and because circumferential actin bundles within epidermal cellsare thought to provide the contractile force for elongation ofthe embryo (Costa et al., 1997; Costa et al., 1998; Priess andHirsh, 1986), we examined the actin pattern in wild-type and mutantembryos with the use of rhodamine-phalloidin to stain filamentousactin. The pharynges of dlg-1(RNAi) terminal-stage embryos, whichappear arrested at the twofold stage (Figure 4H, n = 32/36), lackmost of the radially-oriented actin filaments seen in their twofoldstage (Figure 4E, n = 12/12) and threefold stage (Figure 4F, n= 35/35) wild-type counterparts. We also found that dlg-1(RNAi)worms have fewer than normal circumferential actin bundles, andthe bundles are thicker and often not circumferentially oriented,with variable spacing between the bundles (Figure 4I, n = 24/36).These results suggest that DLG-1 plays an important role in coordinatingactin filaments with the attachment sites at adherens junctionsbetweencells.

HMR-1, HMP-1, and HMP-2 Are Not Required for DLG-1 Localization

What is the function of DLG-1 in the assembly of adherens junctions and the organization of actin filaments? One possibilityis that DLG-1 interacts with the catenin-cadherin system, whichmediates elongation in the C. elegans embryo and includes theproteins HMR-1 (cadherin), HMP-1 ( $alpha$ -catenin), and HMP-2 ( $beta$ -catenin)(Costaet al., 1998). Mutants that lack HMR-1, HMP-1, or HMP-2 recruitAJM-1 to adherens junctions; however, mutant embryos are unableto elongate and possess disorganized actin filaments. To determinewhether DLG-1 requires the catenin-cadherin system for localization,we introduced DLG-1::GFP into mutants that lack these proteins.In elongating and elongated wild-type embryos, DLG-1::GFP is localizedto adherens junctions between cells (Figure 5A,B). Elongatingand terminal-stage embryos that lack HMR-1, HMP-1, and HMP-2 formdisorganized adherens junctions but that still recruit AJM-1 tothese junctions(Costa et al., 1998). Similarly, we find that DLG-1::GFPis localized to adherens junctions in hmr-1 (n = 14/14), hmp-1(n = 15/15), and hmp-2 (n = 28/28) embryos (Figure 5E-H,). Incontrast, DLG-1::GFP fails to properly localize to adherens junctionsin embryos that lack LET-413, which is required for proper apical-basolateralpolarity (Figure 5C, n = 26/26).

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Figure 5. DLG-1:: GFP localization to adherens junctions does not require the cadherin-catenin system. Embryos expressing DLG-1:: GFP (A-H) and HMP-1:: GFP (I-J). Wild-type tadpole (A) and threefold stage (B) embryos localize DLG-1:: GFP to adherens junctions. (C) In contrast, let-413 mutant embryos localize DLG-1:: GFP to punctate structures between cells. (D) Tadpole stage hmr-1 embryos are disorganized but localize DLG-1:: GFP to adherens junctions. Tadpole (E) and terminal (threefold equivalent) stage (F) hmp-1 embryos localize DLG-1:: GFP to their disorganized adherens junctions. Tadpole (G) and terminal (threefold equivalent) stage (H) hmp-2 embryos localize DLG-1:: GFP to their disorganized adherens junctions. HMP-1:: GFP is found at adherens junctions of tadpole stage embryos from both wild-type (I) and dlg-1(RNAi) (J) embryos. Scale bar represents 10 µm.

HMR-1 cadherin is thought to recruit HMP-2 $beta$ -catenin to adherens junctions, and HMP-2 $beta$ -catenin is thought to recruit HMP-1 $alpha$ -catenin to adherens junctions. Thus, mutants that lack HMR-1or HMP-2 protein fail to localize a HMP-1::GFP fusion to adherensjunctions(Costa et al., 1998). We examined the localization ofHMP-1::GFP in dlg-1(RNAi) mutants to determine if DLG-1 is requiredfor HMP-1 recruitment to adherens junctions. HMP-1::GFP is localizedto adherens junctions both in hypodermis (our unpublished results)and intestinal epithelia (Figure 5I,J) in wild-type (n = 37/37)and dlg-1(RNAi) mutant (n = 25/25) embryos, demonstrating thatDLG-1 is not required for HMP-1 localization. These results suggestthat DLG-1 plays an important role in organizing underlying actinthat might be independent of cadherin-cateninsignaling.

DLG-1 Is Involved in Targeting Cypin to Adherens Junctions

Recently, Firestein and colleagues (Firestein et al., 1999) reported the cloning of cypin, a cytosolic PSD-95 interactor,which is involved in MAGUK protein targeting at neuronal synapses.Mammalian cypin is also localized to the basolateral membraneof intestinal epithelial cells (Firestein et al., 1999), whereit can act as an enzyme involved in guanine metabolism and, hence,uric acid production and excretion (Yuan and Atchison, 1999).Since cypin acts to regulate the targeting of MAGUK proteins inmammalian cells, we asked whether CPI-1, a cypin-like moleculein C. elegans (predicted sequence F38E11.3), plays a homologousrole in the targeting of DLG-1 to adherens junctions. We foundthat CPI-1 localizes to the adherens junctions of pharynx (Figure6B) and epidermis (Figure 6E), as evidenced by colocalizationwith DLG-1 in wild-type animals (n = 25/27). No CPI-1 stainingwas detected in cpi-1(RNAi) embryos, indicating that anticypinantibodies specifically detect CPI-1 (n = 17/17, our unpublishedresults). In contrast to wild-type embryos, CPI-1 was mislocalizedin dlg-1(RNAi) embryos, where it was found in small clusters (Figure6H, n = 36/38). This result is surprising, as cypin acts as aregulator of MAGUK targeting in mammalian cells. Instead, theMAGUK DLG-1 actually regulates CPI-1 targeting in vivo in C. elegans.As such, DLG-1 acts to assemble complexes at the adherens junctionas well as to regulate proper adherens junction assembly itself.

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Figure 6. DLG-1 is required to localize CPI-1. Embryos immunostained with anti-PSD-95 antibodies to detect DLG-1 (green, A, D, G) and anticypin antibodies to detect CPI-1 (red, B, E, H). DLG-1 (green) and CPI-1 (red) colocalize to the adherens junctions of wild-type intestine (A-C) and epidermis (D-F). However, in dlg-1(RNAi) embryos, CPI-1 is found in small clusters (arrowheads) along the adherens junctions of intestine (not shown) and epidermis (G-I). Merged images (C, F, I, L, O) contain a 10 µm scale bar.

To assess the role of CPI-1 in adherens junction assembly, we removed CPI-1 expression with the use of RNAi. Surprisingly,these embryos showed normal adherens junction assembly (n = 19/19,our unpublished results) and DLG-1 localization. Thus, CPI-1 mayact as a signaling molecule or enzyme at adherens junctions (Yuanand Atchison, 1999), but it is not required for proper adherensjunction assembly under laboratoryconditions.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Bossinger and colleagues have shown that the PDZ-domain protein DLG-1 is required for the formation of complete and continuousadherens junctions between epithelial cells (Bossinger et al.,2001). Embryos with reduced levels of DLG-1 form adherens junctionswith discontinuous accumulations of the cell junction proteinAJM-1. We have found that nematodes that are fed bacteria thatexpress double-stranded dlg-1 RNA have undetectable levels ofDLG-1 protein (Figure 2H), even when DLG-1 is overexpressed bya transgene (our unpublished results). Using this technique, wehave extended the dlg-1(RNAi) studies by determining that DLG-1is required for the initial localization of AJM-1 to adherensjunctions. We do not believe that the defects in adherens junctionassembly in dlg-1(RNAi) embryos are due to gross defects in cellpolarity and protein trafficking because we find that representativeapical and basolateral proteins are properly localized. Rather,we think that DLG-1 plays a relatively specific role in assemblingadherens junction proteins. This is a novel observation for aMAGUK protein because other members of this family (like DLG andZO-1) have a more general role in cell polarity and the formationof tightjunctions.

Adherens junctions form belt-like structures around epithelial cells, thereby allowing cells to adhere to each other to formsheets. Some of the most well studied components of adherens junctionsinclude cadherin, $alpha$ -catenin, and $beta$ -catenin, encoded by the geneshmr-1, hmp-1, and hmp-2 in C. elegans. Mutations in these genesresult in embryos that fail to elongate and fail to organize theiractin cytoskeleton, a phenotype similar to that of dlg-1(RNAi)mutants(Costa et al., 1998). We have shown that circumferentialactin bundles, which are required for nematode elongation, arenot properly organized with respect to the adherens junctionsin dlg-1(RNAi) embryos. Thus, embryos that lack DLG-1 cannot generatesufficient contractile force and therefore fail to elongate. Ourresults suggest that DLG-1 might function in a previously unknownmechanism (in addition to that of cadherins and catenins) by whichactin filaments are attached to and regulated by adherens junctionsduring the morphological movements of cells. Indeed, other MAGUKproteins have been shown to bind to actin/spectrin-binding protein4.1 family members or complex with cortactin through GKAP andShank (Cohen et al., 1998; Jons et al., 1999; Marfatia et al.,1994; Marfatia et al., 1996; Naisbitt et al., 1999). Our resultsshow that a MAGUK protein, DLG-1, is required for the proper organizationof the actin cytoskeleton, and raise the possibility that thebinding observed between MAGUK proteins and actin-binding proteinsis important for cytoskeletal organization in othersystems.

One simple explanation for the dlg-1(RNAi) phenotype could be that DLG-1 is required to recruit HMR-1, HMP-1, and HMP-2 toadherens junctions. Our results show that localization of $alpha$ -cateninHMP-1, which requires HMR-1 and HMP-2, does not seem to requireDLG-1 (Figure 4). Conversely, DLG-1 localization to adherens junctionsdoes not require HMR-1, HMP-1, or HMP-2 (Figure 4). Could DLG-1function redundantly with the cadherin-catenin system? Doublemutant embryos of dlg-1(RNAi) with hmr-1, hmp-1, or hmp-2 arrestin development at the twofold stage and are indistinguishablefrom dlg-1(RNAi) single mutants; thus, DLG-1 and the cadherin-cateninsystem do not appear to be working synergistically, at least basedon the current morphological and molecular markers available (ourunpublished results). Rather, both DLG-1 and the cadherin-cateninsystem appear to be essential but independent components of epithelialadherensjunctions.

We have sequenced the complete DLG-1 cDNA and have found that DLG-1 is most similar to SAP97, a MAGUK found at synaptic connectionsin the brain and cellular junctions of epithelia. In particular,we have found that the amino termini of DLG-1 and SAP97 are conservedand appear to play a pivotal role in directing DLG-1 localizationto adherens junctions. This is in contrast to Drosophila DLG,which is localized to septate junctions through its second PDZdomain and a unique HOOK region found between the SH3 and GK domains(Thomas et al., 2000). The amino-terminus of other MAGUKs havealso been found to act as subcellular localization signals; forexample, the amino-terminus of PSD-95 is palmitoylated to allowits membrane association(Topinka and Bredt, 1998). Presumablyby dedicating a unique localization domain independent of theother protein-protein interactions domains, MAGUKs can facilitatetheir own localization while maintaining the maximum number ofvalences for other bindingpartners.

It is currently unclear how the amino-terminus of DLG-1 and SAP97 direct their localization within cells. One possibilitywould be an interaction with elements of the actin cytoskeleton.However, mutants for hmr-1, hmp-1, and hmp-2 have severely disorganizedactin networks but are able to localize DLG-1 to adherens junctions,making any role for actin in DLG-1 localization unclear at best.Presumably, further in vivo analysis of DLG-1 localization willshed light on thisissue.

	ACKNOWLEDGMENTS

We thank J. Hardin, M. Labouesse, A. Fire, Y. Kohara, Y. Tabuse, C. Mello, and T. Stiernagle/C. elegans Genetics Center forproviding plasmids, antibodies, and strains. We thank the C. elegansgenome sequencing consortium for providing sequence. We also thankV. Starovoytov and R. Triemer for assistance with the EM analysis.We are grateful to M. Driscoll for critical comments on themanuscript.

	FOOTNOTES

Corresponding author. E-mail address: rongo{at}waksman.rutgers.edu

^§ Both authors contributed equally to thiswork.

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TOP
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DISCUSSION
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