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Address correspondence to Stanley Froehner, Department of Physiology and Biophysics, University of Washington, Seattle, WA 98195-7290. Tel.: (206) 543-0950. Fax: (206) 685-0619. E-mail: froehner{at}u.washington.edu
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Abstract |
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Key Words: syntrophin; aquaporin; dystrophin complex; neuronal nitric oxide synthase; PDZ domain
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Introduction |
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Interest in the syntrophins was originally prompted by the observation that syntrophin was associated with dystrophin and other members of the dystrophin protein family, including utrophin and dystrobrevin (Butler et al., 1992, Ahn and Kunkel, 1995, Dwyer and Froehner, 1995, Yang et al., 1995). Mutations in the dystrophin gene lead to Duchenne and Becker muscular dystrophies (Hoffman et al., 1987). Syntrophins bind to two sites located in the COOH-terminal region of dystrophin such that two syntrophins can attach to one dystrophin (Newey et al., 2000). Dystrophin also binds to dystrobrevin, a protein-containing sequence homology with dystrophin (Sadoulet-Puccio et al., 1996; Peters et al., 1998) and which can also bind two syntrophins (Newey et al., 2000). Thus, the dystrophin complex can bind up to four syntrophins, providing a scaffold for multiple functionally interdependent signaling proteins.
-Syntrophin is the predominant syntrophin isoform in skeletal and cardiac muscle. In skeletal muscle,
-syntrophin is present on the sarcolemma of all fibers, whereas ß1-syntrophin is present on the sarcolemma of only fast type II fibers (Peters et al., 1997). Skeletal muscle ß2-syntrophin is found at high levels only at the postsynaptic membrane of the neuromuscular junctions (Peters et al., 1994; Kramarcy and Sealock, 2000).
2-Syntrophin is also found in skeletal muscle where it has been reported to be located at the sarcolemma (Piluso et al., 2000).
The second PH domain and the highly conserved SU domain are required for interaction with dystrophin (Ahn and Kunkel, 1995; Kachinsky et al., 1999). This leaves the NH2-terminal PH domain and its embedded PDZ domain free to interact with other ligands and thereby link them to the dystrophin complex. Indeed, several molecules have been shown to bind these domains. The NH2-terminal PH domain can bind to phosphatidyl inositol-4,5-bisphosphate (Chockalingam et al., 1999). In vitro biochemical experiments have shown that the PDZ domain of -syntrophin can bind to neuronal nitric oxide synthase (nNOS) (Brenman et al., 1996), muscle voltage-activated sodium channels (Gee et al., 1998a; Schultz et al., 1998), and stress-activated protein kinase-3 (Hasegawa et al., 1999). The ß2-syntrophin PDZ domain binds to microtubule-associated serine/threonine kinase, and the related syntrophin-associated serine/threonine kinase (Lumeng et al., 1999). Diacylglycerol kinase
associates with the PDZ domain of
1-syntrophin (Hogan et al., 2001). Discovery of these interactions has led to the proposal that syntrophins' function is to link signaling molecules to the dystrophin protein complex.
Generation and characterization of -syntrophinnull mice have further strengthened this conclusion. Although the absence of
-syntrophin does not result in discernable musclular dystrophy (Kameya et al., 1999; Adams et al., 2000), the neuromuscular junctions of these mice are structurally aberrant, have reduced levels of acetylcholine receptors and acetylcholine esterase, and are missing utrophin, an ortholog of dystrophin (Adams et al., 2000). Furthermore, nNOS is lost from the sarcolemma in these mice, perhaps due to the absence of the syntrophin PDZ domain.
In addition to nNOS, the water channel, aquaporin-4, also shows dependence on -syntrophin for sarcolemmal localization. Aquaporin-4 is absent from the sarcolemma when
-syntrophin is missing either due to the loss of the entire dystrophin complex in the mdx mouse (Frigeri et al., 1998) or specific loss of
-syntrophin by targeted gene disruption (Yokota et al., 2000). Aquaporins are responsible for the high membrane permeability of water in many different tissues, including kidney, brain, and the gastrointestinal tract (Frigeri et al., 1995). Aquaporin-4 is an integral membrane protein present in the sarcolemma of fast twitch fibers, although its physiological role in muscle is unknown. The COOH terminus of aquaporin-4 contains a likely PDZ domain interaction sequence, -VLSSV. However, this sequence is not one that we would expect a priori to bind syntrophin PDZs based on the published consensus binding sequences (Gee et al., 1998a, 1998b). Thus, the functional relationship between the
-syntrophin PDZ domain and sarcolemmal aquaporin-4 expression is unknown.
PDZ domains are involved in the assembly of macromolecular complexes at numerous sites of membrane specialization. These specializations include the neuromuscular synapse (Adams et al., 2000), synapses between neurons in the brain (Sheng, 1996; Kornau et al., 1997), the apical and basoloateral membranes of polarized epithelia (Short et al., 1998; Kachinsky et al., 1999), and receptor-dense areas that induce apoptosis in tumor cells (Yanagisawa et al., 1997). The most common mode of interaction is between the COOH-terminal tail of ligand and the PDZ domain (Doyle et al., 1996), although association with internal PDZ binding sequences and PDZ-PDZ heterodimerization also occurs (Gee et al., 1998b; Hillier et al., 1999; Tochio et al., 2000). Despite the fact that PDZ proteins have been studied extensively and the structure is known in great detail (Hillier et al., 1999), the PDZligand interactions have not been characterized in vivo. An in vivo demonstration is important for two reasons. First, other interactions have been proposed to play a role in the localization of nNOS to the membrane by -syntrophin. (Venema et al., 1997; Abdelmoity et al., 2000). The relative importance of these multiple binding sites has yet to be determined. Second, and perhaps more important, the large number of PDZ-containing proteins and potential binding proteins undoubtedly requires a level of specificity that extends beyond that achieved by the amino acid sequence adjacent to the terminal S-X-V motif. We observed such specificity with the PDZ domain of ß1-syntrophin that can bind nNOS in vitro (Gee et al., 1998a), but that is unable to recruit nNOS to the sarcolemma in vivo in the absence of
-syntrophin (Adams et al., 2000). The development of in vivo systems for the study of this and similar phenomena will be very important in understanding how specificity of the formation of the complexes is governed, and to what extent the interactions found in vitro actually exist in the cell.
These issues have prompted us to develop mouse models to test the function of the -syntrophin PDZ interactions in vivo. We have developed lines of transgenic mice that express a form of
-syntrophin in which the PDZ domain has been replaced with an epitope tag. We have used this transgenic line in combination with one expressing full-length
-syntrophin in dominant negative and genetic rescue experiments. These new mouse models demonstrate that nNOS and aquaporin-4, but not sodium channels, require the presence of an
-syntrophin PDZ domain for sarcolemmal localization in vivo. Furthermore,
-syntrophin requires the presence of the dystrophin complex to form a stable association with the sarcolemma.
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Results |
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Generation and characterization of transgenic mice
We developed two lines of transgenic mice (Fig. 1). The first, Tg -Syn, expresses full-length
-syntrophin. The second, Tg
PDZ, expresses an altered form of
-syntrophin in which the PDZ domain was replaced with the hemagglutinin (HA) epitope tag. The expression of both proteins is under control of the mouse muscle creatine kinase promoter; therefore, they are expressed primarily in skeletal and cardiac muscle. Endogenously produced
-syntrophin can be differentiated from the
PDZ transgene product by the use of a monoclonal antibody (1351) that recognizes an epitope within the PDZ domain (Materials and methods). Both transgene products and endogenous
-syntrophin are recognized by rabbit polyclonal antibody, SYN17, as the antibody was made to a peptide sequence that lies just downstream of the PDZ domain. Immunoblot analysis using these antibodies shows that proteins derived from the transgenes are expressed at levels 2030-fold higher than endogenous
-syntrophin in skeletal muscle (Fig. 1 B).
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Tg PDZ protein also displaces ß1-syntrophin (Fig. 2). Sarcolemmal labeling for ß1-syntrophin is greatly reduced in the Tg
PDZ muscle, but neighboring blood vessels, where the transgene is not expressed, show normal high levels of expression. The Tg
-Syn protein does not displace ß1-syntrophin to the same extent as the Tg-
PDZ protein, despite being expressed at somewhat higher levels (Fig 1 B). Sarcolemmal levels of ß1-syntrophin are reduced in the muscles of the Tg
-Syn mice, but are still clearly present and even brightly labeled on the smaller fibers. These small fibers may represent areas of immature muscle. ß1-Syntrophin is expressed in most skeletal muscle fibers during the first six weeks of mouse muscle development after which its sarcolemma levels decline in all but the fast type II fibers (Kramarcy and Sealock, 2000). Other than having a higher number of small fibers, muscles of the transgenic mice did not show any of the abnormalities commonly found in dystrophic muscle (central nuclei, split fibers, fibrosis, etc.).
Association of transgenic syntrophins with dystrophin
Syntrophin associates with the sarcolemma by binding directly to dystrophin and dystrobrevin (Ahn and Kunkel, 1995, Dwyer and Froehner, 1995, Yang et al., 1995; Newey et al., 2000). To determine if the transgenic syntrophins Tg PDZ and Tg
-Syn bound dystrophin, we isolated the dystrophin complex from muscle homogenates by immunoprecipitation with anti-dystrophin antibody. Immunoblotting of the complexes with anti-HA antibody showed that the Tg
PDZ protein copurified with dystrophin (Fig. 3). Similar blotting with SYN17 confirmed the presence of Tg
PDZ and also showed that Tg
-Syn copurified with dystrophin as expected (Fig. 3). We consistently observed proportionally more Tg
PDZ than either the endogenous or transgenic full-length syntrophin in the dystrophin isolates (Fig. 3), suggesting that the Tg
PDZ syntrophin may have a higher affinity for dystrophin than the full-length forms. This conclusion is consistent with the immunofluorescence data (Fig. 2) showing that Tg
PDZ syntrophin displaced ß1-syntrophin to a greater extent than did Tg
-Syn.
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PDZ ligand restoration in syntrophin-null/transgenic crosses
In genetically modified mice lacking -syntrophin, nNOS is absent from the sarcolemma (Kameya et al., 1999; Adams et al., 2000). This has been assumed to be due to the loss of the
-syntrophin PDZ domain. We tested this assumption directly by breeding the two syntrophin transgenic mice lines onto the
-syntrophinnull background. Immunofluorescence studies show that the sarcolemmal localization of nNOS is "rescued" by the full-length syntrophin transgene but not by the
PDZ transgene (Fig. 6). Thus, in vivo, nNOS localization to the sarcolemma depends on the presence of an
-syntrophin PDZ domain. Similarly, aquaporin-4, normally absent from the sarcolemma of
-syntrophinnull mice, was restored by the full-length transgene but not by the
PDZ construct (Fig. 6). Our attempts to show in vitro that the aquaporin-4 COOH-terminal sequence binds directly to
-syntrophin have been unsuccessful, even under conditions in which a similar peptide corresponding to the COOH terminus of the sodium channel binds robustly (unpublished data). Nevertheless, these in vivo data clearly show that sarcolemmal localization of aquaporin-4 requires the
-syntrophin PDZ domain.
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Discussion |
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Some PDZ-ligands have been characterized in vivo using invertebrate models. In Caenorhabditis elegans, three PDZ proteins, Lin-2, Lin-7, and Lin-10, mediate the localization of the LET-23 receptor (Kaech et al., 1998). This receptor fails to localize to the basolateral surface when the PDZ proteins are mutated. Mutational studies in Drosophila show that the PDZ domaincontaining protein, discs large, is required for the neuromuscular junction localization of Shaker potassium channels (Tejedor et al., 1997). However, no direct test of PDZ-ligand interactions has been reported in whole animal mammalian systems. In this paper, we have described one approach that should be generally applicable to in vivo analyses in a broad range of systems.
We investigated the functional role of the -syntrophin PDZ domain in vivo by using a dominant-negative approach. We developed a transgenic mouse line that expresses a PDZ-less form of
-syntrophin at high levels in skeletal muscle. The observation that
PDZ
-syntrophin is localized to the sarcolemma indicates that the PDZ domain is not required for plasma membrane association. This result is consistent with the demonstration that the PH2 and SU domains in tandem are required for binding to dystrophin and other family members (Ahn and Kunkel, 1995; Kachinsky et al., 1999). Furthermore, the
PDZ form of
-syntrophin competed with endogenous
-syntrophin for binding sites on the sarcolemma (dystrophin and dystrobrevin). This competition produced skeletal muscle that contained little or no sarcolemmal syntrophin PDZ domain as demonstrated by the reduction in labeling with mAb 1351, an antibody that binds to an epitope within the PDZ domain of
-syntrophin.
In addition to displacing endogenous -syntrophin, the
PDZ
-syntrophin was able to displace ß1-syntrophin from the sarcolemma as well. These data suggest that
- and ß1-syntrophin compete for the same binding sites, at least under conditions of high
-syntrophin expression, to facilitate membrane association. Interestingly, the
PDZ form was more effective than the full-length Tg
-syntrophin in displacing ß1-syntrophin. This suggests that the absence of the PDZ domain increases the affinity of syntrophin for dystrophin/dystrobrevin. Thus, the PDZ domain of syntrophin may act to regulate the interaction of syntrophin with the dystrophin complex. An interesting possibility is that binding of a ligand to the PDZ domain promotes association of the PH-SU domains with their binding sites on dystrophin. Such regulation is similar to that demonstrated for MAGUK family proteins (McGee and Bredt, 1999) and could be important for localizing PDZ ligands to the sarcolemma via the dystrophin complex.
Two syntrophin PDZ ligands have been studied extensively in vitro. nNOS and voltage-gated sodium channels bind to -syntrophin PDZ domains but via different mechanisms. nNOS contains a beta-finger immediately adjacent to its own PDZ domain that interacts directly with the PDZ domain of syntrophin (Hillier et al., 1999). In contrast, sodium channels bind to syntrophin PDZ domains via the more conventional COOH terminal "SXV" motif (Gee et al., 1998a). The function of this interaction is unknown, but syntrophin binding could potentially affect the ion conduction properties of the sodium channel or mediate its participation in a scaffold involving other channels and/or modifying enzymes. However, our data show that syntrophin binding is not required for normal sodium channel distribution on the sarcolemma. This conclusion is in agreement with the observation that sodium channel density is only slightly reduced in skeletal muscle of the mdx mouse which lacks dystrophin and, therefore, sarcolemmal syntrophin (Ribaux et al., 2001).
In contrast, sarcolemmal localization of nNOS does depend on the presence of an -syntrophin PDZ domain. In the absence of a sarcolemmal syntrophin PDZ domain, nNOS fails to localize to the sarcolemma. The localization of nNOS to the sarcolemma is important in regulating blood flow in skeletal muscle during muscle activity. Thomas et al. (1998) have shown that in the absence of nNOS, attenuation of adrenergically stimulated vasoconstriction does not occur. Similar results were obtained from mdx mice which lack sarcolemmal nNOS (Thomas et al., 1998). Therefore, it is likely that the
-syntrophin PDZ domain is not only necessary for proper localization of nNOS but is required for proper function of nNOS in skeletal muscle as well.
In addition to syntrophin, another membrane-associated protein, caveolin-3, has been shown to bind nNOS (Venema et al., 1997). However, in muscle from the Tg PDZ mice and the Tg
PDZ/
-syntrophinnull cross, we could not detect nNOS on the membrane. Therefore, the interaction of nNOS with caveolin-3 must be insufficient for stable retention of nNOS at the sarcolemma. It has also been proposed that nNOS may localize to the sarcolemma by binding membrane-associated proteins directly via its PDZ domain (Abdelmoity et al., 2000). Because in the absence of a syntrophin PDZ domain we do not detect nNOS on the sarcolemma, if such interactions occur they are insufficient for stable retention. Alternatively, such interactions could be induced by association of the nNOS beta finger with the syntrophin PDZ domain.
A third putative ligand for the -syntrophin PDZ domain is aquaporin-4. Aquaporin-4 is normally present on the sarcolemma of fast twitch fibers of skeletal muscle but is absent from muscle that lacks the dystrophin protein complex (Frigeri et al., 1998). The COOH-terminal amino acid sequence of aquaporin-4 is -VLSSV, a potential class I PDZ domain interaction sequence. Therefore, we used our transgenic mice to determine if the membrane localization of aquaporin-4 depended on a syntrophin PDZ domain. In the absence of an
-syntrophin PDZ domain, aquaporin-4 is also absent from the sarcolemma. Aquaporin-4 is an integral membrane protein that contains six transmembrane domains and therefore does not need to be recruited to the sarcolemma like the soluble protein, nNOS. Rather, the syntrophin PDZ domain is likely involved in targeting or stabilizing aquaporin-4.
The in vivo studies presented here also provide insight into how -syntrophin interacts with the sarcolemma. Data from the Tg
PDZ show that
-syntrophin is localized to the sarcolemma and binds directly to dystrophin in the absence of a PDZ domain. However, the immunofluorescence studies of muscle expressing full-length and
PDZ syntrophin on an mdx background show that, even when expressed at high levels, syntrophin does not associate with the sarcolemma in the absence of dystrophin. Apparently, interactions with sodium channels or phosphatidyl inositols are insufficient to localize syntrophin to the sarcolemma. In fact, our data indicate that interaction with the dystrophin complex is necessary and sufficient for sarcolemmal
-syntrophin localization.
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Materials and methods |
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Mice expressing Tg PDZ and mice expressing Tg
-Syn were bred onto an
-syntrophinnull background by crossing with the previously characterized
-syntrophinnull mice (Adams et al., 2000). Similarly, the transgenic lines were bred onto the mdx background. In each case the genotypes were confirmed by PCR of genomic DNA derived from tail biopsies.
Antibodies
Isoform specific rabbit polyclonal antibodies SYN17 (-syntrophin) and SYN37 (ß1-syntrophin) have been previously characterized (Peters et al., 1997). The polyclonal anti-HA antibody was purchased from Zymed Laboratories, Inc. For detection of nNOS, two antibodies were used: an mAb from BD Transduction Laboratories (San Diego, CA) was used for Western blots, and a polyclonal antibody (Ab) from Diasorin (Stillwater, MN) was used for immunofluorescence microscopy. The polyclonal Ab to aquaporin-4 was purchased from Chemicon. The polyclonal Ab recognizing both the SCN4A and SCN5A isoforms of the sodium channel was a gift from S. Rock Levinson, (University of Colorado Health Sciences Center, Denver, CO). The utrophin polyclonal Ab was raised against a peptide at the COOH terminus identical to that previously described for Ab 1862 (Kramarcy et al., 1994). The mAb Mandra 1, recognizing dystrophin, was purchased from Sigma-Aldrich.
We have previously described mAb 1351 (Froehner et al., 1987) and have shown that it recognizes an epitope within the PDZ domain of -, ß1-, and ß2-syntrophin (Gee et al., 1998a). However, for this study it was important to identify the epitope more specifically. Therefore, we synthesized 29 overlapping peptides of 13 amino acids each that spanned the entire PDZ domain of
-syntrophin (SPOTs blot; Genosys). Incubation of mAb 1351 with these peptides using the protocol supplied by the manufacturer showed that the epitope is confined to a 13amino acid segment with the sequence: ISKIFKGLAADQT. This sequence corresponds to amino acids 108120 within the
-syntrophin PDZ domain.
Immunoblotting
Muscle protein detergent extracts were prepared as previously described (Peters et al., 1997). Dystrophin was isolated by incubating muscle extracts with the dystrophin mAb Mandra-1 followed by precipitation with protein Gcoated beads (Sigma-Aldrich). After washing the beads three times with phosphate buffered saline (10 mM sodium phosphate, 150 mM sodium chloride, pH 7.4), we resuspended the specifically bound protein in SDS-PAGE sample buffer. Protein samples were subjected to electrophoresis on an 8% polyacrylamide tricine-buffered gel. Separated proteins were transferred to Immobilon-P membrane (Millipore Corp.) and incubated with the indicated antibody as previously described (Peters et al., 1997). Bands were visualized using a peroxidase-conjugated secondary antibody (Jackson ImmunoResearch Laboratories) and a luminol-based substrate (Pierce Chemical Co.).
Fluorescence microscopy
Immunofluorescence labeling was performed on unfixed muscle flash frozen in liquid nitrogen cooled isopentane. 8-µm cryosections were incubated with antibody (30 nM IgG, in each case) as described by Peters et al. (1997). Primary antibodies were visualized using Alexa-488 and -568 (Molecular Probes) conjugated secondary antibodies. Sections were analyzed using a Leica TCS NT confocal microscope.
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Footnotes |
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* Abbreviations used in this paper: Ab, antibody; HA, hemagglutinin; nNOS, neuronal nitric oxide synthase; PDZ, PSD-95, discs-large, ZO-1; PH, pleckstrin homology; SU, syntrophin unique region.
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Acknowledgments |
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This work was funded by grants from the Muscular Dystrophy Association (M.E. Adams and S.C. Froehner) and from the National Institutes of Health (NS33145).
Submitted: 29 June 2001
Revised: 10 August 2001
Accepted: 10 August 2001
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References |
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