The E3 Ubiquitin Ligase Atrophin Interacting Protein 4 Binds Directly To The Chemokine Receptor CXCR4 Via a Novel WW Domain-mediated Interaction

Deepali Bhandari^*, Seth L. Robia, and Adriano Marchese^*^,

Departments of Pharmacology and Experimental Therapeutics and Cell and Molecular Physiology and *Program in Molecular Biology, Stritch School of Medicine, Loyola University Chicago, Maywood, IL 60153

Submitted March 21, 2008; Revised November 25, 2008; Accepted December 19, 2008
Monitoring Editor: Thomas Sommer

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The E3 ubiquitin ligase atrophin interacting protein 4 (AIP4)mediates ubiquitination and down-regulation of the chemokinereceptor CXCR4. AIP4 belongs to the Nedd4-like homologous toE6-AP carboxy terminus domain family of E3 ubiquitin ligases,which typically bind proline-rich motifs within target proteinsvia the WW domains. The intracellular domains of CXCR4 lackcanonical WW domain binding motifs; thus, whether AIP4 is targetedto CXCR4 directly or indirectly via an adaptor protein remainsunknown. Here, we show that AIP4 can interact directly withCXCR4 via a novel noncanonical WW domain-mediated interactioninvolving serine residues 324 and 325 within the carboxy-terminaltail of CXCR4. These serine residues are critical for mediatingagonist-promoted binding of AIP4 and subsequent ubiquitinationand degradation of CXCR4. These residues are phosphorylatedupon agonist activation and phosphomimetic mutants show enhancedbinding to AIP4, suggesting a mechanism whereby phosphorylationmediates the interaction between CXCR4 and AIP4. Our data reveala novel noncanonical WW domain-mediated interaction involvingphosphorylated serine residues in the absence of any prolineresidues and suggest a novel mechanism whereby an E3 ubiquitinligase is targeted directly to an activated G protein-coupledreceptor.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The chemokine receptor CXCR4 and its cognate ligand stromalcell-derived factor (SDF)-1 ${alpha}$ (Bleul et al., 1996; Oberlin etal., 1996), also termed CXCL12 (Murphy, 2002), have criticalfunctions in cardiogenesis, vasculogenesis, neural development,stem cell homing, and leukocyte chemotaxis among others (Nagasawaet al., 1996; Tachibana et al., 1998; Zou et al., 1998; Lu etal., 2002). Dysregulation of CXCR4 signaling, expression, orboth is associated with several pathological conditions, includingcardiovascular disease, cancer, and warts, hypogammaglobulinemia,recurrent infection, and myelokathexis (Damas et al., 2000;Muller et al., 2001; Balkwill, 2004; Diaz and Gulino, 2005;Walter et al., 2005). Thus, elucidating the mechanisms thatregulate CXCR4 is critical for understanding its contributionto these pathologies and for developing new strategies to manipulatereceptor signaling to treat diseases associated with CXCR4 dysregulation.

CXCR4 is a G protein-coupled receptor (GPCR) that couples toG ${alpha}$ _i to elicit a variety of cellular signaling responses (Busilloand Benovic, 2007). Similar to other GPCRs, signaling by CXCR4is rapidly desensitized at the cell surface, followed by internalizationinto endosomes in which it is sorted to lysosomes for degradation.The posttranslational modification of CXCR4 with ubiquitin,a 76-amino acid polypeptide, is critical for regulation of CXCR4endocytic trafficking (Marchese and Benovic, 2001). We haveshown previously that CXCR4 ubiquitination on carboxy-terminaltail (C-tail) lysine residues targets the receptor for lysosomaldegradation (Marchese and Benovic, 2001; Marchese et al., 2003).Ubiquitination of activated CXCR4 is mediated by the E3 ubiquitinligase atrophin interacting protein 4 (AIP4) at the plasma membrane(Marchese and Benovic, 2001; Marchese et al., 2003). However,the mechanism by which AIP4 is targeted to activated CXCR4 remainsunknown.

AIP4 is a member of the Nedd4-like family of E3 ubiquitin ligasesand ubiquitinates a diverse set of proteins involved in a varietyof cellular processes (Ingham et al., 2004; Shearwin-Whyattet al., 2006). AIP4 is composed of an amino-terminal C2 domain,a proline-rich region (PRR), four tandemly linked WW domains,and a carboxy-terminal catalytic homologous to E6-AP carboxyterminus (HECT) domain. C2 domains are phospholipid bindingdomains that may also mediate protein–protein interactions(Cho and Stahelin, 2006). The PRR has been shown to bind toSrc homology 3 domains (Angers et al., 2004; Janz et al., 2007).WW domains, named after two conserved tryptophan residues, are $~$ 35–45 amino acid residues in length and are structurallysimilar; they can be divided into four distinct groups basedon their ability to interact with proline-rich sequences invarious contexts (Macias et al., 2002; Hu et al., 2004; Inghamet al., 2005a). Typically, the WW domains mediate binding ofthe Nedd4-like family members with their targets either directlyor indirectly through a protein intermediate (Ingham et al.,2004; Shearwin-Whyatt et al., 2006). All four WW domains ofAIP4 have been shown to bind to PY motifs (e.g., PPxY, PPPY)within their target proteins and/or peptides containing PY motifs(Winberg et al., 2000; Ingham et al., 2005b). The HECT domainis a conserved $~$ 350-amino acid catalytic domain that containsan active site cysteine residue that forms a direct thiolesterbond with ubiquitin before its transfer to target proteins (Huibregtseet al., 1995; Pickart and Eddins, 2004).

The molecular determinants responsible for targeting the ubiquitinationmachinery to GPCRs remain poorly understood. CXCR4 was the firstmammalian GPCR shown to be ubiquitinated by a Nedd4-like E3family member (Marchese et al., 2003). In yeast cells, the ${alpha}$ -matingfactor receptor (Ste2), a GPCR, is ubiquitinated by Rsp5, theyeast ortholog of Nedd4-like E3s (Dunn and Hicke, 2001). Geneticand biochemical studies have revealed that the Rsp5 WW domainsare required for ubiquitination of the receptor, suggestingthat the WW domains are involved in receptor recognition. However,the C-tail of Ste2 lacks any known WW recognition motifs, suggestingthat Rsp5 is recruited to the receptor via an indirect mechanism,possibly via an intermediate protein that is yet to be identified(Dunn and Hicke, 2001). As with Ste2, the intracellular domainsof CXCR4 do not contain obvious WW domain recognition sequences,but whether an adaptor protein is required for AIP4 recruitmentto the receptor remains to be determined. Interestingly, studiesof the mammalian β₂-adrenergic receptor (β₂AR), aprototypic GPCR used widely for studying GPCR signaling andtrafficking (Pierce et al., 2002), implicate the endocytic adaptorprotein arrestin-3 in the recruitment of the E3 ubiquitin ligaseNedd4-1 to the receptor (Shenoy et al., 2001, 2008). Arrestinshave been implicated in the regulation of CXCR4 signaling andtrafficking (Orsini et al., 1999; Cheng et al., 2000); however,recently, we have shown that arrestins are not involved in CXCR4ubiquitination (Bhandari et al., 2007). Thus, whether AIP4 targetingto CXCR4 involves the WW domains either through a direct orindirect interaction and/or possibly other domains remains tobe determined. Here, we report that AIP4 can bind directly toCXCR4 via an interaction between CXCR4 C-tail serine residuesand the WW domains of AIP4 revealing, a novel mechanism wherebyan E3 ligase is directly targeted to a GPCR.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cell Lines, Reagents, and Antibodies
Human embryonic kidney (HEK) 293 cells (Microbix, Toronto, ON,Canada) were maintained in DMEM (Mediatech, Herndon, VA) supplementedwith fetal bovine serum (FBS; HyClone Laboratories, Logan, UT).The anti-hemagglutinin (HA) monoclonal antibodies (mAbs) andpolyclonal antibodies were purchased from Covance (Richmond,CA). The anti-FLAG M2-horseradish peroxidase (HRP) mAb and ${lambda}$ protein phosphatase were from Sigma-Aldrich (St. Louis, MO).The anti-HIS antibody was from QIAGEN (Valencia, CA). The anti-AIP4polyclonal (D-20) and monoclonal (G11) antibodies were fromSanta Cruz Biotechnology (Santa Cruz, CA), whereas the anti-glutathionetransferase (GST) antibody and glutathione-Sepharose 4B resinwere from GE Healthcare (Little Chalfont, Buckinghamshire, UnitedKingdom). The anti-β-tubulin mAb was from Accurate Chemical& Scientific (Westbury, NY), and the anti-actin antibodywas from MP Biomedicals (Solon, OH). Horse anti-mouse and anti-goatantibody horseradish conjugates and VECTASHIELD mounting mediumfor immunofluorescence were from Vector Laboratories (Burlingame,CA). The Alexa-Fluor 594 goat anti-mouse conjugate was fromInvitrogen (Carlsbad, CA). Stromal cell-derived factor (SDF)-1 ${alpha}$ (a.k.a. CXCL12) was from PeproTech (Rocky Hill, NJ). Calf intestinalalkaline phosphatase (CIP) was from New England Biolabs (Ispwich,MA).

DNA Constructs
HA-tagged CXCR4, FLAG-AIP4, and FLAG-ubiquitin were as describedpreviously (Marchese et al., 2003). GST-fusion constructs ofthe four individual AIP4 WW domains were as described previously(Marchese and Benovic, 2004) and kindly provided by Dr. AnthonyPawson (Samuel Lunenfeld Research Institute, Toronto, ON, Canada).The HA-tagged serine mutants of CXCR4 in pcDNA3 were generatedby the polymerase chain reaction (PCR) by using HA-CXCR4 WTas the template. For GST-fusion constructs of the C-tail, wild-type,S324/5A, and S324/5D CXCR4 were used as templates to amplifyamino acid residues 308-352 by PCR and cloned in-frame to GSTby using the pGEX-4T2 bacterial expression vector. For GST-fusionconstructs of AIP4, wild-type AIP4 (amino acids 2-862), andWW domains I–IV (wild-type and mutant constructs; aminoacids 260-486) were amplified by PCR and cloned into the BamHIand XhoI sites of pGEX-4T2 to generate full-length GST-AIP4and GST-WW-I-IV. Individual point mutants of AIP4 were madein the context of GST-WW-I-IV to include Q297A, N329A, Q297A/N329A,W313A, W345A, W313A/W345A, and Q297A/N329A/W313A/W345A (4A).To create amino-terminally tagged His-AIP4 and His-WW-I-IV (wild-typeand point mutants), full-length AIP4 (amino acids 2-862) andWW domains I–IV (amino acids 260-486) were amplified byPCR and subcloned into the BamHI-PvuII and BamHI-XhoI sitesof pRSET-A (Invitrogen), respectively. The HA-CXCR4-YFP construct(described in Bhandari et al., 2007) was used as the templateto clone the HA-S324/325A-yellow fluorescent protein (YFP) mutant.Full-length AIP4 was amplified and subcloned into the KpnI-BamHIsites of pECFP-N1 (Clontech, Mountain View, CA) plasmid to generateAIP4-cyan fluorescent protein (CFP). The integrity of all theconstructs was verified by sequencing.

GST-Fusion Protein Expression and Binding Assay
Escherichia coli BL21 cells transformed with GST-fusion constructswere grown overnight at 37°C. The next day, cultures werediluted 1:50 and grown to an OD₆₀₀ $~$ 0.4 at 37°C and theninduced with 0.1 or 0.5 mM isopropyl β-D-thiogalactoside(IPTG) for 1–3 h at 18°C. Cells were pelleted andresuspended in binding buffer (20 mM Tris-HCl, pH 7.4, 150 mMNaCl, 0.1% Triton X-100, 1 mM dithiothreitol, 10 µg/mlleupeptin, 10 µg/ml pepstatin A, and 10 µg/ml aprotinin),and sonicated on ice. Lysates were clarified by centrifugationat 21,000 x g for 20 min at 4°C, followed by incubationwith glutathione-Sepharose 4B resin for 1 h at 4°C whilerocking, and then they were washed and resuspended in bindingbuffer. For binding experiments, GST-fusion proteins ( $~$ 0.3–1µg) were incubated with cell lysates prepared from HEK293cells expressing the protein of interest or purified His-taggedproteins for 4–16 h. Samples were washed in binding buffer,eluted in 2x sample buffer for 30 min at room temperature andanalyzed by SDS-polyacrylamide gel electrophoresis (PAGE) followedby Western blotting.

Expression and Purification of 6xHis-AIP4
E. coli BL21-DE3 cells, transformed with 6xHis-AIP4- and 6xHis-WW-I-IV-pRSET-Awere grown to an OD₆₀₀ 0.3–0.5 and induced with 1.0 mMIPTG for 1–4 h at 18°C. Cells were pelleted and resuspendedin lysis buffer (for 6xHis-AIP4, the buffer used was 50 mM phosphatebuffer, pH 7.4, 300 mM NaCl, and 10 mM imidazole; for 6xHis-WW-I-IVthe buffer used was 50 mM phosphate buffer, pH 8.0, 500 mM NaCl,10 mM imidazole, and 0.1% Triton X-100) containing proteaseinhibitors (aprotinin, pepstatin A, and leupeptin, each at 10µg/ml), sonicated on ice, and clarified by centrifugation.Clarified lysates containing 6xHis-AIP4 were applied to preequilibratednickel-nitrilotriacetic acid mini columns, washed (wash buffer:50 mM phosphate buffer, pH-7.4, 300 mM NaCl, and 30 mM imidazole),and eluted (elution buffer: 50 mM phosphate buffer, pH 7.4,300 mM NaCl, and 300 mM imidazole), according to the manufacturer'sinstructions (ProPur IMAC Mini spin column kit; Nalge Nunc International,Rochester, NY). Clarified lysates containing 6xHis-WW-I-IV (WTand point mutants) were incubated with equilibrated His-SelectNi-affinity beads (Sigma-Aldrich) for 1 h at 4°C, washed,and eluted in the same buffer as the lysis buffer containing100–500 mM imidazole. The binding assay between 6xHis-AIP4(500 ng) or various amounts of 6xHis-WW-I-IV and GST-C-tailwas as described above.

Ubiquitination Assay
For detection of ubiquitinated CXCR4, HEK293 cells were transientlytransfected using FuGENE-6 transfection reagent with DNA encodingHA-tagged CXCR4 and FLAG-tagged ubiquitin. Cells were treatedwith CXCL12 (100 nM) for 30 min followed by immunoprecipitationof CXCR4 and immunoblotting to detect incorporated ubiquitin,essentially as described previously (Marchese and Benovic, 2001;Marchese et al., 2003).

Fluorescence Resonance Energy Transfer (FRET) Experiments
Fluorescence imaging was performed using an inverted microscopeequipped with a 1.49 numerical aperture (NA) objective, anda back-thinned camera (iXon 887; Andor Technology, Belfast,Northern Ireland). The detector was cooled to –100°C,by using a recirculating liquid coolant system (Koolance, Auburn,WA). Image acquisition and acceptor photobleaching were automatedwith custom software macros in MetaMorph (Molecular Devices,Sunnyvale, CA) that controlled motorized excitation/emissionfilter wheels (Sutter Instrument, Novato, CA) with filters forCFP and YFP (Semrock, Rochester, NY). HEK293 cells transientlytransfected with cDNAs encoding HA-CXCR4-YFP and AIP4-CFP wereplated onto poly-L-lysine–coated chambered borosilicatecoverglass (Nalge Nunc International). The cells were serumstarved for 1 h before measuring the FRET between HA-CXCR4-YFPand AIP4-CFP, and they were maintained in the same serum-freemedium throughout the course of the experiment. FRET betweenHA-CXCR4-YFP and AIP4-CFP was measured both in the absence andpresence of 100 nM CXCL12 at 20–23°C by using theacceptor photobleaching method (Kenworthy, 2001; Kelly et al.,2008). For measuring FRET in the presence of CXCL12, acceptorphotobleaching was started 10 min after the manual additionof CXCL12. The progressive photobleaching protocol was as follows:100-ms acquisition of CFP image, 40-ms acquisition of YFP image,followed by a 10-s exposure to selectively photobleach YFP (504/12-nmexcitation). The apparent FRET efficiency was calculated fromthe fluorescence intensity of the CFP (427/10-nm excitation)donor before and after acceptor-selective photobleaching, accordingto the formula %FRET = [1 – (F_prebleach/F_postbleach)]x 100.

Coimmunoprecipitation Assay
HEK293 cells transiently coexpressing FLAG-AIP4 and HA-CXCR4or pcDNA3.0 were serum starved for 3–4 h and stimulatedwith either vehicle (DMEM + 0.5% FBS) or 30 nM CXCL12 for 15min. Cells were washed once with ice-cold phosphate-bufferedsaline (PBS) and lysed in ice-cold buffer (20 mM Tris-Cl, pH7.5, 150 mM NaCl, 1% Triton X-100, protease inhibitors [10 µg/mleach pepstatin, leupeptin, and aprotinin], and phosphatase inhibitorcocktails I and II [Sigma-Aldrich]). Cell lysates were sonicated,clarified by centrifugation at 21,000 x g for 20 min at 4°C,and CXCR4 was immunoprecipitated using a polyclonal anti-HAantibody. Immunoprecipitates were analyzed for the presenceof FLAG-AIP4 by SDS-PAGE followed by immunoblotting.

Total Internal Reflection Fluorescence (TIRF) Microscopy Experiments
HEK293 cells transiently coexpressing HA-CXCR4 wild-type, S324/5A,or S324/3D and AIP4-CFP were passaged onto poly-L-lysine (0.1mg/ml)–coated coverglass chambers (Nalge Nunc International).The next day, cells were serum starved with DMEM containing20 mM HEPES for at least 1 h before starting the experimentand maintained in the same medium at 20–23°C throughoutthe course of the experiment. TIRF imaging was performed witha Nikon TE2000-U inverted microscope. Illumination from a 449-nmdiode laser (RGBlase) was introduced through a Nikon TIRF IIilluminator, reflected with a multiple band dichroic mirror(Chroma Technology, Rockingham, VT), and directed to the sampleusing a 1.49 NA objective. Images were obtained using a filter(Semrock) for CFP (472/30 nm), a computer-controlled emissionfilter wheel (Sutter Instrument), and an electron-multiplying-charge-coupleddevice camera (iXon 887; Andor Technology) cooled to –100°Cwith a recirculating liquid coolant system (Koolance). Imageacquisition was automated with custom software macros in MetaMorph(Molecular Devices). Time-lapse images were obtained every 5s for 10 min. After the first 15 images, the acquisition waspaused briefly and resumed after addition of 100 nM CXCL12 tothe cell chamber. Images were analyzed and processed using ImageJ1.3v software (National Institutes of Health, Bethesda, MD).To calculate the area of the basal plasma membrane in contactwith the coverslip, TIRF images were autothresholded and analyzedwith the ImageJ macro "Analyze particles." The image stack wasthen manually thresholded to select puncta, and particles ofsize 0.05–1.0 and circularity 0.5–1.0 were countedwith the Analyze particles macro. This analysis yielded themean density (puncta per square micrometer) before and afterCXCL12 stimulation.

Determination of CXCR4 Phosphorylation by Confocal Immunofluorescence Microscopy by Using a Custom Phosphoserine-specific Antibody
A custom mAb that recognizes dually phosphorylated serine residues324 and 325 was obtained from A and G Pharmaceutical (Baltimore,MD). The antibody was raised against the following keyhole limpethemocyanin-conjugated peptide: SRG-pS-pS-LKILSKGKR (pSer324-pSer325).Supernatants from 28 hybridomas were initially screened againstbovine serum albumin (BSA)-conjugated phosphorylated and unphosphorylatedpeptides by enzyme-linked immunosorbent assay (SupplementalFigure S3). Subsequently, supernatants from 17 hybridomas wereused to screen HEK293 cells expressing HA-tagged CXCR4 and S324/5Aby Western blotting (with dilutions up to 1:10), immunoprecipitationand confocal immunofluorescence microscopy. Although the dataobtained by Western blotting and immunoprecipitation were inconclusive,one clone (5E11), which recognizes phospho-peptide S324/5 butnot unphosphorylated peptide as determined by enzyme-linkedimmunosorbent assay, was found to recognize doubly phosphorylatedCXCR4 on serine residues 324 and 325 by confocal immunofluorescencemicroscopy. HEK293 cells transfected with wild-type HA-CXCR4-YFPor S324/5A mutant were passaged onto poly-L-lysine–coatedcoverslips. After 48 h, cells were serum starved for 3–4h in DMEM containing 20 mM HEPES, pH 7.4, followed by replacementwith the same medium containing either vehicle (0.1% BSA inPBS) or ligand (30 nM CXCL12) for 5, 15, or 30 min. Cells werethen washed with PBS, fixed with 3.7% formaldehyde-PBS solutionfor 15 min, and permeabilized with 0.01% saponin-PBS for 10min at room temperature. Cells were incubated with 5% FBS in0.01% saponin-PBS for 30 min at 37°C followed by immunostainingwith clone 5E11 (hybridoma supernatant, 1:10 dilution) at 37°Cfor 30 min. Cells were washed and incubated with Alexa-Fluor563-conjugated secondary antibody at 37°C for 30 min. Finally,cells were washed and fixed with 3.7% formaldehyde-PBS beforemounting onto glass slides using VECTASHIELD mounting medium.

For CIP and ${lambda}$ phosphatase treatments, cells were fixed and permeabilizedfollowed by incubation with either 200 U of CIP (New EnglandBiolabs) at 37°C or 400 U of ${lambda}$ phosphatase (Sigma-Aldrich)at 30°C for 1 h. Control cells were incubated under similarconditions in the respective buffers only. Cells were washedwith PBS and subject to blocking and subsequent staining andmounting steps as described above. Images were acquired usingan LSM-510 laser scanning confocal imaging system (equippedwith a 1.4-megapixel cooled extended spectral range RGB digitalcamera; Carl Zeiss, Thornwood, NY) with a C-Apo 40x/1.2 waterobjective at 512 x 512 resolution. Acquired images were analyzedusing ImageJ 1.3v software.

Degradation Assay
Agonist promoted degradation of HA-CXCR4 WT and the serine mutantswas detected by immunoblot analysis, as described previously(Marchese et al., 2003).

Statistical Analysis
One-way analysis of variance (ANOVA) and Student's t test wereperformed using GraphPad Prism version 4.00 for Macintosh (GraphPadSoftware, San Diego CA; www.graphpad.com). Two-way ANOVA wasperformed using GraphPad Prism and GB-STAT (Dynamic Microsystems,Silver Spring, MD).

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

AIP4 Binds Directly to CXCR4
The machinery responsible for ubiquitinating GPCRs remains poorlydefined. We have shown that the E3 ubiquitin ligase AIP4 mediatesagonist-promoted ubiquitination of the chemokine receptor CXCR4at the plasma membrane and functions in endosomal sorting totarget the receptor for lysosomal degradation (Marchese et al.,2003). Although AIP4 colocalizes with CXCR4 at the plasma membraneupon agonist treatment, the determinants targeting AIP4 to CXCR4remain unknown (Marchese et al., 2003). Because lysine residueswithin the C-tail of CXCR4 are the sites for ubiquitin modification,we first assessed whether AIP4 interacted with the C-tail ofCXCR4. Whole cell lysates prepared from HEK293 cells expressingFLAG-tagged AIP4 were incubated with the C-tail of CXCR4 fusedto GST (Figure 1A) immobilized on glutathione-Sepharose resin,and bound AIP4 was detected by immunoblotting. As shown in Figure 1B,AIP4 bound to GST-C-tail but not to GST alone, suggesting thatAIP4 interacts with the C-tail of CXCR4. To determine whetherthe interaction is direct or mediated by an AIP4-associatedprotein, we examined the binding of purified HIS-tagged full-lengthAIP4 to GST-C-tail. As shown in Figure 1C, purified HIS-AIP4showed a substantial amount of binding to GST-C-tail, comparedwith GST alone, indicating that the interaction between CXCR4and AIP4 is direct.

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Figure 1. The carboxy-terminal tail of CXCR4 interacts with AIP4. (A) Schematic representation of the carboxy-terminal tail of CXCR4 fused to GST. CXCR4 is a seven transmembrane domain spanning integral plasma membrane protein. The predicted cytoplasmic carboxy-terminal tail (amino acid residues 308-352) was fused to GST to create GST-C-tail. (B) The C-tail of CXCR4 interacts with AIP4. Whole cell lysates from HEK293 cells expressing FLAG-tagged AIP4 were incubated with GST-C-tail (57 nM) or GST (71 nM) alone. Input represents 0.4% of the lysate used in the binding reactions. Immunoblot was probed with the anti-FLAG M2 antibody to detect FLAG-AIP4. Blot was stained with Ponceau-S to determine the levels of the GST proteins used in the binding assay. Data from one of three independent experiments are shown. (C) The C-tail of CXCR4 binds directly to AIP4. Histidine-tagged AIP4 (HIS-AIP4; $~$ 5.2 pmol) was incubated with GST-C-tail (57 nM) or GST (71 nM) alone. Input represents $~$ 0.2% of the purified HIS-tagged AIP4 used in the binding assay. Immunoblot was probed with an anti-HIS antibody to detect HIS-AIP4. A GelCode blue stained gel indicating the levels of the GST proteins used in the binding assay is shown. Data from one of three independent experiments are shown.

We next wanted to determine whether CXCR4 and AIP4 interactin cells upon agonist activation by coimmunoprecipitation. HEK293cells transiently expressing HA-CXCR4 and FLAG-AIP4 were treatedwith vehicle or 30 nM CXCL12 for 15 min followed by immunoprecipitationof HA-CXCR4 and immunoblotting to determine the presence ofFLAG-AIP4 in the immunoprecipitates. As shown in Figure 2A,coimmunoprecipitation of AIP4 with CXCR4 was enhanced upon agonisttreatment compared with vehicle-treated cells, indicating thatCXCL12 treatment promoted the interaction between CXCR4 andAIP4. To further characterize the interaction, we used FRETcoupled with fluorescence microscopy, which are powerful techniquesto measure protein–protein interactions in live cells(Piston and Kremers, 2007

). To this end, CXCR4 and AIP4 weretagged with fluorescent proteins YFP and CFP, respectively,which when in proximity can undergo FRET (Piston and Kremers,2007

). YFP was placed at the carboxy terminus of HA-CXCR4, whichdoes not interfere with its internalization and traffickingto lysosomes upon agonist stimulation (Bhandari et al., 2007

).AIP4 was tagged with CFP at its carboxy terminus, which doesnot seem to interfere with its activity (Supplemental Figure1). To measure FRET between HA-CXCR4-YFP and AIP4-CFP, we followedan acceptor-selective photobleaching protocol as described previously(Kelly et al., 2008

). HEK293 cells were transiently transfectedwith HA-CXCR4-YFP and AIP4-CFP and FRET was monitored in thepresence or absence of 100 nM CXCL12. Images from a representativecell treated with CXCL12 showing prebleach and postbleach YFPand CFP fluorescence are shown in Figure 2B. YFP fluorescencewas selectively photobleached (Figure 2B, bottom), which ledto enhanced CFP fluorescence, compared with prebleach fluorescence,indicating FRET between HA-CXCR4-YFP and AIP4-CFP (Figure 2B,top). The increased CFP fluorescence was observed at the cellperiphery and in a perinuclear intracellular pool, reflectingthe plasma membrane and an endosomal pool, compartments in whichwe have shown previously that CXCR4 and AIP4 colocalize (Marcheseet al., 2003

). Figure 2C shows the time-dependent change inCFP emission intensity from cells treated with (n = 17) or without(n = 20) CXCL12, while undergoing progressive and complete photobleachingof YFP (data not shown). The AIP4-CFP emission significantlyincreased upon treatment of cells with CXCL12 compared withcells that were not treated with CXCL12 (unpaired Student'st test, p < 0.0001), suggesting an enhanced association betweenHA-CXCR4-YFP and AIP4-CFP compared with untreated cells. Thereforetaken together, our data indicate that agonist activation promotesthe interaction between CXCR4 and AIP4.

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Figure 2. Agonist mediated interaction between CXCR4 and AIP4. (A) Agonist enhances the interaction between CXCR4 and AIP4. Serum-starved HEK293 cells cotransfected with FLAG-AIP4 and HA-CXCR4 or pcDNA3.0 were treated with either vehicle (DMEM containing 0.5% FBS) or CXCL12 (30 nM) for 15 min. The clarified whole cell lysates (WCL) were immunoprecipitated (IP) by using an anti-HA antibody and analyzed by SDS-PAGE and immunoblotting to detect bound FLAG-AIP4. Immunoprecipitates were also immunoblotted (IB) for HA-CXCR4 and WCL were immunoblotted to detect the expression of FLAG-AIP4 and HA-CXCR4. The HA antibody in the CXCR4 IP recognizes multiple bands, which are likely differentially glycosylated forms of the receptor. Immunoblots were stripped and reprobed for actin to assess loading. The bar graph represents average FLAG-AIP4 binding normalized to the level of receptor in the IPs. Error bars represent the SEM from three independent experiments. Binding of FLAG-AIP4 to CXCR4 in the presence of CXCL12 was significantly increased over its binding to the unstimulated receptor. *p < 0.05, unpaired t test. (B) FRET analysis of fluorescent protein-tagged CXCR4 and AIP4 in live cells. Shown are images of a representative cell treated with CXCL12. Prebleach and postbleach donor (HA-CXCR4-YFP; yellow) and acceptor (AIP4-CFP; cyan) images are shown. Arrows indicate cell periphery where FRET was observed. (C) In total, 20 cells without CXCL12 (–) and 17 cells with CXCL12 (+) treatment were analyzed from three independent experiments. The average F/F₀ ratio for AIP4-CFP, where F₀ and F are the donor emissions before and after progressive photobleaching, respectively, is plotted against time. Fluorescence intensity was measured using the whole cell for the analysis. The error bars represent the SE. The data were subject to an unpaired t test (p < 0.0001).

AIP4 WW Domains Are Critical for Binding to CXCR4
To further understand the mechanism of the interaction betweenAIP4 and CXCR4, we next sought to identify the determinantsresponsible for the direct binding between AIP4 and CXCR4. Althoughthe WW domains of AIP4 have been shown to interact with proline-rich(i.e., PY) motifs within target proteins (Winberg et al., 2000

;Ingham et al., 2005a

), there is some suggestion that they mayinteract with noncanonical motifs (Ingham et al., 2005a

). Therefore,although the C-tail of CXCR4 does not contain proline residues,to understand the molecular basis for the interaction betweenCXCR4 and AIP4, we initially examined whether the WW domainsof AIP4 mediate the interaction with CXCR4. Full-length AIP4(GST-AIP4) and the four tandemly linked WW domains (GST-WW-I-IV)were expressed as GST fusion proteins (Figure 3A), purifiedon glutathione-Sepharose resin, and incubated with whole celllysates prepared from cells expressing HA-CXCR4 and bound receptorwas detected by immunoblotting. As shown in Figure 3B, CXCR4bound to full-length GST-AIP4 as expected; and surprisingly,CXCR4 also bound to GST-WW-I-IV. To determine whether otherregions of AIP4 could also bind to CXCR4, we created a GST-fusionprotein in which the WW domains were deleted (GST-AIP4 ${Delta}$ WW) andtested the ability of this mutant to bind to CXCR4. As shownin Figure 3C, CXCR4 binding to GST-AIP4 ${Delta}$ WW was significantlydiminished compared with GST-AIP4 and GST-WW-I-IV, suggestingthat the WW domains represent the main CXCR4 binding region.To confirm that the WW domain mediated interaction was not viaan intermediate protein, we next performed the binding experimentsusing purified proteins. As shown in Figure 3D, GST-C-tail boundto increasing amounts of purified HIS-tagged WW-I-IV, indicatinga direct interaction between the C-tail of CXCR4 and the WWdomains of AIP4. Thus, our data reveal that AIP4 WW domainsinteract directly with the C-tail of CXCR4, likely through anovel noncanonical recognition sequence.

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Figure 3. The WW domains of AIP4 mediate the interaction with CXCR4. (A) Schematic representation of AIP4. AIP4 has a C2 domain, a PRR, four tandemly linked WW domains, and a catalytic HECT-domain. GST was fused to the amino terminus of full-length AIP4 (GST-AIP4), to AIP4 lacking the WW domains (GST-AIP4 ${Delta}$ WW) and to the WW domains alone (GST-WW-I-IV). (B and C) CXCR4 interacts with the WW domains of AIP4. (B) Whole cell lysates (WCL) from HEK293 cells transiently expressing HA-CXCR4 and empty vector (pcDNA3) were incubated with 1 µg of GST-AIP4, GST-WW-I-IV, or GST alone. (C) WCL from HEK293 cells stably expressing HA-CXCR4 were incubated with equimolar amounts ( $~$ 22 pM) of GST-AIP4, GST-AIP4 ${Delta}$ WW, GST-WW-I-IV, or GST alone. Samples were resolved by SDS-PAGE, followed by immunoblotting with an anti-HA antibody (top) to detect bound HA-CXCR4. Coomassie- (B) and GelCode blue (C)-stained gels (bottom) indicate the level of the GST fusion proteins used in the binding experiments. Input represents $~$ 0.6% (B) and 0.2% (C) of the lysate that was used for the binding experiment. Data from one of three experiments are shown. Receptor levels were determined by densitometry and average receptor binding was expressed as the percentage of control wild-type AIP4 binding (WT) ± SEM from three independent experiments (C, right). Please note that the SEM for ${Delta}$ WW binding is ± 0.39. Data were analyzed by a one-way ANOVA, followed by Bonferroni's post hoc test. Binding to the ${Delta}$ WW mutant was significantly different from WT and WW-I-IV binding. *p < 0.05. (D) The C-tail interacts directly with AIP4 WW domains. Increasing amounts of HIS-tagged WW-I-IV were incubated with equal amounts of GST-C-tail or GST alone. Bound HIS-WW-I-IV (60% of sample) was detected by immunoblotting with a HIS antibody conjugated to HRP. A known amount of HIS-WW-I-IV (3 ng) was also immunoblotted. The asterisk represents nonspecific binding of the HIS-HRP antibody to GST-C-tail. HIS-WW-I-IV binding was determined by densitometric analysis and normalization to GST-C-tail levels. Data are the mean HIS-WW-I-IV binding ± SE from four experiments. The data were analyzed by a one-way ANOVA followed by Bonferoni's post hoc test; p < 0.05 between 100 and 500 ng.

WW domains are characterized by the presence of two conservedtryptophan residues and are thought to adopt a similar structure;however, their recognition sequence preferences may differ (Zarrinparand Lim, 2000

). Therefore, to gain further mechanistic insightinto the interaction, we wanted to determine the ability ofeach of the four individual WW domains of AIP4 to interact withCXCR4. The four WW domains were expressed individually as GST-fusionproteins and assessed for their ability to bind HA-CXCR4 expressedin HEK293 cells. As shown in Figure 4A, CXCR4 bound to GST-WW-Iand GST-WW-II, but not to GST-WW-III and GST-WW-IV, indicatingthat the interaction with CXCR4 is specific to WW domains Iand II. Interestingly, binding to individual WW domains I andII was not as great as that observed with binding to WW-I-IVor full-length AIP4, suggesting higher avidity of binding whenthe WW domains are tandemly linked, and consistent with thepossibility that AIP4 may bind to two CXCR4 molecules throughsimultaneous interactions via both WW domains I and II. Regardless,our data indicate that CXCR4 has a preference for WW domainsI and II, via a novel noncanonical recognition sequence.

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Figure 4. Identification of residues within WW domains I and II that are critical for binding to CXCR4. (A) CXCR4 interacts with AIP4 WW domains I and II. Whole cell lysates (WCL) from HEK293 cells expressing HA-CXCR4 were incubated with GST alone ( $~$ 110 nM), GST-AIP4 ( $~$ 25 nM), GST-WW-I-IV ( $~$ 55 nM) or GST fusions of each of the four individual WW domains ( $~$ 100 nM). Immunoblot was probed with an anti-HA antibody to detect bound HA-CXCR4. A Coomassie-stained gel is shown to indicate the level of GST proteins used in the binding assay. Input represents 1.5% of the lysate used in the binding assay. Shown are data from one of three independent experiments. (B) Alignment of the WW domains from AIP4 and several members of the Nedd4-like family of E3 ligases. The four WW domains of AIP4 are shown aligned. Residues that are either identical or conserved to both WW domains I and II are high-lighted black. Residues that are unique to each of the four WW domains are boxed and shaded gray. Sequence of the Pin1 WW domain is also shown and the critical arginine residue shown to be important for phosphorylation mediated binding to Pin1 is shaded. The WW domains from other members of the Nedd4-like HECT domain family are shown (WWP1, WWP2, Nedd-4, and Rsp5). The conserved tryptophan residues from which the WW domain derives its name are boxed. A space (-) has been inserted to maximize the alignment. The three conserved β sheets that are connected by two loops are indicated above the sequence. Residues are numbered relative to their appearance in the full-length protein. The single-letter amino acid code is used. Sequences were obtained from the GenBank flat files under the following accession numbers: NP_113671 (AIP4), AAC51324 (WWP1), AAC51325 (WWP2), NP_011051 (yeast RSP5), P46934 (hNedd4), and AAC50492 (Pin1). (C–E) Identification of critical residues within WW domains I and II important for binding to CXCR4. WCL from HEK293 cells expressing HA-CXCR4 were incubated with the indicated GST-WW domain fusion protein ( $~$ 25–50 nM) or GST ( $~$ 45 nM) alone. The immunoblot (IB) was probed with an anti-HA antibody to detect bound receptor (top). IB was stripped and reprobed with an anti-GST antibody (C and E) or gel was stained with GelCode blue (D) to reveal level of GST fusion proteins used in the assay. Input represents 0.3% of the lysate used in the binding assay. Bound receptor levels were determined by densitometry and average receptor binding was expressed as the percentage of control GST-WW-I-IV wild-type (WT) binding ± SEM from three (D and E) or 5 (C) independent experiments. Data were analyzed by either a t test (E) or a one-way ANOVA and Bonferroni's post hoc test (C and D). Binding of the double mutants (W313/W345A and Q297/N329A) and the quadruple mutant (W313/Q297/W345/N329A) to CXCR4 was significantly different from wild-type binding. C, *p < 0.01; D, *p < 0.05; and E, *p < 0.011. (F) Purified HIS-tagged WWI-IV WT, Q297/N329A, W313/W345A, and 4A ( $~$ 70 nM) were incubated with equimolar amounts of either GST-C-tail WT or GST alone. Immunoblot was probed with an anti-HIS antibody to detect HIS-WWI-IV. The input represents $~$ 2% of the purified His-WWI-IV (WT or mutants) used in the binding assay. The immunoblot was stripped and reprobed with an anti-GST antibody to detect the levels of GST proteins used in the binding assay. HIS-WWI-IV binding was determined by densitometric analysis, and data represent the mean ± SE from three independent experiments. Data were analyzed by a one-way ANOVA and Bonferroni's post hoc test. The binding of HIS-WWI-IV mutants to GST-C-tail was significantly different from that of wild-type (WT). *p < 0.01.

To characterize the interaction further, we next wanted to identifythe residues within WW domains I and II that are important forthe interaction. Typically, the second conserved tryptophanresidue within WW domains forms part of the binding pocket thatenables interactions with proline-based recognition sequencesof target proteins (Zarrinpar and Lim, 2000

). For AIP4 WW domainsI and II, the second conserved tryptophan residue correspondsto Trp313 and Trp345, respectively (Figure 4B). To assess whetherthese residues are also involved in the interaction with CXCR4,we mutated Trp313 and Trp345 to alanine either together or alonewithin the context of GST-WW-I-IV and then assessed the abilityof the GST-fusion proteins to bind to HA-tagged CXCR4 expressedin HEK293 cells. As shown in Figure 4C, the extent of HA-CXCR4binding to GST-WW-I-IV containing individual point mutations(W313A or W345A) was somewhat diminished compared with wild-typeGST-WW-I-IV binding. However, binding of HA-CXCR4 to the doublemutant (W313A/W345A) was significantly reduced by $~$ 60% comparedwith wild-type binding. Together, these data indicate that conservedresidues Trp313 and Trp345 within WW domains I and II, respectively,are important for CXCR4 recognition, although the mechanismfor the interaction remains to be determined.

Because we still observed significant binding to the doubletryptophan mutant, it is likely that other residues within theWW domains contribute to the interaction with CXCR4. Multipleresidues are known to be important for standard WW domain andproline-based interactions (Verdecia et al., 2000; Kasanov etal., 2001). To identify such residues, we aligned the aminoacid sequence of the four AIP4 WW domains to each other to determinewhether we could identify amino acid residues unique to WW domainsI and II, but not III and IV, because we reasoned that theseresidues were likely to be important for the specificity inbinding of the WW domains (Figure 4B). Using this strategy,we identified two conserved residues, Gln297 and Asn329, inthe loop region that connects the first β sheet with thesecond β sheet of WW domains I and II, respectively (seeFigure 4B for sequence). Interestingly, these residues are locatedat the analogous position to an arginine residue that has beenshown to be important for binding of group IV WW domains tophospho-serine/threonine-Pro [p(Ser/Thr)] motifs (Verdecia etal., 2000). To determine whether Gln297 and Asn329 are importantfor binding to CXCR4, we changed them to alanine residues withinthe context of GST-WW-I-IV either together or alone and testedthe ability of these fusion proteins to bind to HA-tagged CXCR4expressed in HEK293 cells. As shown in Figure 4D, binding ofHA-CXCR4 to the single GST-WW-I-IV point-mutants (Q297A andN329A) was similar to that observed with wild-type GST-WW-I-IV.However, binding of HA-CXCR4 to the double mutant (Q297A/N329A)was significantly reduced (by $~$ 58%; p < 0.05) compared withits binding to wild-type GST-WW-I-IV, suggesting that Gln297and Asn329 are important for binding HA-CXCR4. We next determinedthe effect of combining the tryptophan mutations with the glutamineand asparagine mutations (W313/W345/Q297/N329A or 4A) on thebinding of WWI-IV to CXCR4. As shown in Figure 4E, when allfour residues were simultaneously changed to alanine residues,binding to CXCR4 was almost abolished, suggesting that theseresidues are important for mediating the interaction with CXCR4.To ensure that these WW domain residues are indeed mediatingthe direct interaction with the tail of CXCR4 we further examinedthe interaction using purified proteins. As shown in Figure 4F,binding of GST-C-tail to HIS-WW-I-IV double mutants (Q297A/N329Aand W313A/W345A) and the quadruple mutant (4A) was significantly(p < 0.01) attenuated compared with wild-type HIS-WW-I-IV,further indicating that the C-tail of CXCR4 interacts directlywith AIP4 WW domains involving residues Q297, N329, W313, andW345.

CXCR4 C-Tail Serine Residues Mediate the Interaction with AIP4
The C-tail of CXCR4 seems to be the major site for AIP4 bindingand ubiquitination, however the critical residues that mediatethis interaction are not known. Interestingly, in previous studieswe have shown that CXCR4 C-tail serine residues 324, 325, and330 are important for agonist-promoted receptor degradation(Marchese and Benovic, 2001). However, the mechanistic basisfor their role in CXCR4 degradation remains unknown. One possibilityis that these serine residues are important for mediating AIP4binding and thus subsequent ubiquitination and degradation ofthe receptor. To this end, we first examined whether CXCR4 C-tailserine residues mediate binding to AIP4 by testing the abilityof GST-WW-I-IV to bind to CXCR4 serine mutant receptors S324/5Aand S330A (Figure 5A). Whole cell lysates prepared from HEK293cells expressing HA-tagged wild-type CXCR4 or C-tail mutantswere incubated with GST-WW-I-IV or GST alone and bound receptorswere detected by immunoblotting. As shown in Figure 5, B andC, GST-WW-I-IV binding to the S324/5A CXCR4 mutant was significantlyreduced by $~$ 67% compared with its binding to wild-type receptor.In contrast, binding to S330A mutant was similar to wild-typereceptor binding, suggesting that this serine residue is notinvolved in AIP4 binding. These findings suggest that serinesresidues S324/5 within the C-tail of CXCR4 are important forbinding to the WW domains of AIP4.

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Figure 5. CXCR4 C-tail serine residues mediate the interaction with AIP4. (A) CXCR4 C-tail amino acid sequence. Shown is the amino acid sequence of the carboxy-terminal tail of CXCR4 and the various serine receptor mutants. The single-letter amino acid code is used. (B and C) CXCR4 serine receptor mutant binding to AIP4. (B) Whole cell lysates (WCL) from HEK293 cells expressing wild-type HA-CXCR4 and the indicated serine mutants were incubated with GST-WW-I-IV ( $~$ 17 nM) or GST ( $~$ 97 nM) alone. Bound receptor was detected by immunoblotting (top). Blots were stripped and reprobed with an anti-GST antibody (bottom). Input represents 0.3% of the lysate used in the binding assay. Shown are representative blots. (C) Bound receptor levels were determined by densitometry and average receptor binding was expressed as the percentage of control CXCR4 binding ± SEM from five independent experiments. Data were analyzed by a Kruskal–Wallis one-way ANOVA, followed by Dunn's post hoc test. Binding to S3245A was significantly different from WT and S330A binding. *p < 0.05. (D) FRET analysis between S324/5A and AIP4. Cells expressing HA-S324/5A-YFP and AIP4-CFP were treated and the FRET efficiency was calculated as described in Materials and Methods. Shown is the average FRET efficiency between HA-S324/5-YFP and AIP4-CFP from cells treated with (n = 23) or without (n = 26) CXCL12. Data from Figure 2 were used to calculate the FRET efficiency between HA-CXCR4-YFP and AIP4-CFP. Data were analyzed by a two-way ANOVA (p < 0.01), followed by a Bonferroni's post hoc test (*p < 0.0001, between CXCL12 treated wild-type and S324/5A cells).

To determine the importance of these serine residues in mediatingan interaction with AIP4 in live cells, we examined the interactionbetween S324/5A and AIP4 via FRET analysis. HEK293 cells transientlytransfected with HA-S324/5A-YFP and AIP4-CFP were either treatedor not treated with CXCL12 and FRET was monitored using theacceptor photobleaching protocol described above. The averageFRET efficiency between HA-S324/5A and AIP4-CFP in the absenceof CXCL12 treatment was 9.3% (n = 26), which was similar tothe average FRET efficiency in the presence of CXCL12 treatment(10.8%; n = 23), suggesting that agonist fails to enhance theinteraction between S324/5A and AIP4 (Figure 5D). This is incontrast to what we observed with wild-type CXCR4. We calculatedthe FRET efficiency from the data in Figure 2, in which we examinedthe interaction between HA-CXCR4-YFP and AIP4-CFP. In this case,the average FRET efficiency was 10.3% in the absence of CXCL12,which increased significantly (p < 0.001) to 16.7% in thepresence of CXCL12, indicating that agonist enhances the interactionbetween CXCR4 and AIP4 (Figure 5D). Interestingly, FRET alsooccurred in the absence of agonist, suggesting that CXCR4 andAIP4 interact constitutively. We also observed similar amountsof FRET under basal conditions with S324/5A compared with wild-typeCXCR4 (9.3 vs. 10.3% for S324/5A and wild-type CXCR4, respectively).This is in contrast to the GST-WW-I-IV interaction studies inwhich there was a decreased level of binding to S324/5A comparedwith wild-type receptor, even though these experiments wereperformed in the absence of agonist treatment (Figure 5B). Itis possible that coexpression of fluorescent protein-taggedreceptors and AIP4 contributes to a high degree of constitutiveassociation that is not dependent on serine residues 324 and325. Nevertheless, upon treatment with agonist, a significantincrease in the FRET efficiency ( $~$ 62%) was observed only betweenwild-type receptor and AIP4 and not between the mutant receptorand AIP4, suggesting that serine residues 324 and 325 are criticalfor mediating the agonist promoted interaction between CXCR4and AIP4 in cells.

We have previously shown that AIP4 mediates agonist-promotedubiquitination and degradation of CXCR4 (Marchese et al., 2003)and that serine residues 324 and 325 are critical for mediatingagonist promoted degradation of CXCR4 (Marchese and Benovic,2001). To determine whether these serine residues are also importantfor CXCR4 ubiquitination, we assessed the ubiquitination statusof the S324/5A mutant. HEK293 cells transfected with HA-taggedwild-type CXCR4 or S324/5A, plus FLAG-tagged ubiquitin weretreated with agonist for 30 min followed by receptor immunoprecipitationand immunoblotting to detect incorporation of ubiquitin, essentiallyas described previously (Marchese and Benovic, 2001). As shownin Figure 6A, agonist treatment failed to promote ubiquitinationof the S324/5A mutant compared with wild-type CXCR4, which isconsistent with the inability of this mutant to interact withAIP4 and undergo agonist promoted degradation (Figure 6B; Marcheseand Benovic, 2001). To determine the relative contribution ofserine residues 324 and 325 on agonist-promoted degradationof CXCR4, we examined the ability of the individual S324A andS325A mutants to undergo agonist promoted degradation. As shownin Figure 6B, the degradation of the individual mutants (S324Aand S325A) was modestly affected compared with the S324/5A doublemutant, suggesting that both residues are needed for mediatingagonist-promoted degradation of CXCR4. Thus, together our datasuggest that the recruitment of AIP4 through its interactionwith serine residues 324 and 325 within the C-tail of CXCR4is critical for receptor ubiquitination and degradation.

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Figure 6. CXCR4 C-tail serine residues 324 and 325 are important for CXCR4 ubiquitination and degradation. (A) Ubiquitination of S324/5A is attenuated compared with wild-type CXCR4. HEK293 cells were transfected with the indicated CXCR4 constructs and FLAG-tagged ubiquitin. Cells were treated in the presence or absence of 100 nM SDF for 30 min at 37°C, followed by immunoprecipitation (IP) of the receptor and immunoblotting (IB) to detect the incorporation of epitope-tagged ubiquitin. Blots were then stripped and reprobed with an anti-HA mAb to assess receptor levels. Shown are representative blots from one of six independent experiments. Ubiquitinated CXCR4 levels were assessed by densitometric analysis and the –fold increase upon CXCL12 treatment compared with vehicle treatment was normalized to receptor levels present in the immunoprecipitates. Ubiquitination of CXCR4 was significantly increased compared with the S324/5A mutant. Unpaired t test: *p < 0.03. (B) Involvement of serine residues 324 and 325 in agonist-promoted degradation of CXCR4. HEK293 cells transfected with the indicated HA-tagged CXCR4 constructs were treated in the presence or absence of 10 nM SDF for 3 h at 37°C in DMEM containing 10% FBS and 50 µg/ml cycloheximide, essentially as described previously (Marchese and Benovic, 2001

). Equal amounts of lysates were subject to SDS-PAGE and immunoblotting to detect receptor levels. Receptor levels were assessed by densitometric analysis and normalized to tubulin levels. The bars represent the average percent receptor degraded in cells treated with agonist compared with vehicle-treated cells from five independent experiments. Error bars represent the SE of the mean.

CXCR4 Phosphorylation Is Important for AIP4 Binding
Because serine residues are potential sites of phosphorylation,we next wanted to investigate the role of CXCR4 phosphorylationin AIP4 recruitment. We generated phosphomimetic mutants ofHA-CXCR4 by mutating serine residues 324 and 325 to asparticacid (Figure 7A) and tested the ability of these receptor mutantsexpressed in HEK293 cells to bind to GST-WW-I-IV and GST alone.As shown in Figure 7B, binding of the individual aspartic acidmutants S324D and S325D and the double aspartic acid mutantS324/5D to GST-WW-I-IV was enhanced compared with wild-typeCXCR4. Similarly, binding of purified HIS-WW-I-IV to GST-C-tail-S324/5Dwas enhanced, whereas binding to the S324/5A mutant was decreased,compared with the wild-type C-tail (Figure 7C). Consistent withthe increased ability of the S324/5D mutant to bind to the WWdomains of AIP4, degradation of S324/5D was significantly enhancedcompared with wild-type receptor at an early time point (30min) after agonist treatment (Figure 7D). Together, our datasuggest that a negative charge located at positions 324 and325 can promote the CXCR4/AIP4 interaction and receptor degradation.

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Figure 7. CXCR4 phospho-mimetic mutants show enhanced binding to AIP4. (A) The amino acid sequence of the carboxy-terminal tail of CXCR4 and the various serine-to-aspartic acid receptor mutants. (B) CXCR4 phospho-mimetic mutant binding to GST-WW-I-IV. Whole cell lysates from HEK293 cells expressing wild-type HA-CXCR4 or the indicated serine mutants were incubated with GST-WW-I-IV ( $~$ 12 nM) or GST ( $~$ 38 nM) alone. Immunoblot was probed with an anti-HA antibody to detect bound receptor. Shown is an immunoblot to indicate the level of the GST proteins used in the binding assay. Input represents 0.3% of lysate used in the binding assay. Receptor levels were determined by densitometry and average receptor binding was expressed as the percentage of control CXCR4 binding ± SEM from four independent experiments. (C) Binding analysis using purified proteins. Purified HIS-tagged WW-I-IV ( $~$ 70 nM) was incubated with equimolar amounts of either the wild-type C-tail, S324/325A, and S324/325D fused to GST or GST alone. Immunoblot was probed with an anti-HIS antibody to detect bound HIS-WW-I-IV. The input represents $~$ 1% of the purified His-WWI-IV used in the binding assay. The immunoblot was stripped and reprobed with an anti-GST antibody to detect the levels of GST proteins used in the binding assay. HIS-WWI-IV binding was determined by densitometric analysis, and data represent the mean ± SE from three independent experiments. (D) Enhanced agonist-promoted degradation of CXCR4 phospho-mimetic mutant S324/5D. Degradation of HA-tagged CXCR4 was assessed in cells treated with 10 nM SDF for 30 min at 37°C, essentially as described previously (Marchese and Benovic, 2001

). The bars represent the average percentage of receptor degraded in cells treated with agonist compared with vehicle-treated cells from four independent experiments. Error bars represent the SE of the mean. Degradation of S324/5D was significantly enhanced as compared with wild-type receptor degradation (average mean, 3.8 vs. 27.2%). Unpaired t test, *p < 0.03.

We next investigated whether these serine residues are indeedphosphorylated upon receptor activation by generating a custommAb (clone 5E11) that recognizes simultaneous phosphorylationof serine residues 324 and 325 (pS³²⁴pS³²⁵). Cells were treatedwith CXCL12 for 15 min and the phosphorylation status of CXCR4was assessed by confocal immunofluorescence microscopy by usingclone 5E11. As shown in Figure 8, A and B, CXCR4 was robustlyphosphorylated on serine residues 324 and 325 upon treatmentwith CXCL12 for 15 min but not in vehicle-treated cells (0.1%BSA in PBS). Notably, 5E11 staining completely overlapped withYFP-tagged CXCR4 only at the cell surface and not on intracellularreceptor (Figure 8B, yellow in merged panel), suggesting thatthese residues were simultaneously phosphorylated at the cellsurface and dephosphorylated before or once CXCR4 appeared onendosomes. To confirm that 5E11 recognizes serine residues 324and 325, we assessed the ability of 5E11 to immunostain themutant S324/5A upon agonist treatment. As shown in Figure 8,C and D, 5E11 failed to recognize the S324/5A mutant expressedto similar levels as the wild-type receptor, confirming thatserine residues 324 and 325 are part of the epitope recognizedby 5E11. Also, of note, cells that did not express CXCR4 werenot reactive to 5E11 (Figure 8B), further confirming the specificityof this antibody toward CXCR4. To confirm that 5E11 recognizesphosphorylated CXCR4, we examined the staining pattern of 5E11in cells expressing wild-type CXCR4 that were treated with agonistfollowed by incubation with ${lambda}$ phosphatase, alkaline phosphatase,or buffer alone. Under these conditions, 5E11 was nonimmunoreactivein cells treated with lambda phosphatase and alkaline phosphatase(Figure 8, E and F), but not in cells treated with buffer alone(data not shown), suggesting that CXCR4 was dephosphorylatedand that 5E11 indeed recognizes phosphorylated CXCR4. Together,these data indicate that CXCR4 is simultaneously phosphorylatedon serine residues 324 and 325 at the plasma membrane upon activationwith CXCL12.

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Figure 8. CXCR4 C-tail serine residues 324 and 325 are phosphorylated upon agonist activation. HEK293 cells transiently expressing HA-tagged CXCR4-YFP (A, B, E, and F) or S324/5A-YFP (C and D) were incubated with either vehicle or CXCL12 for 15 min. Cells were fixed, permeabilized, and immunostained using an anti-phosphoserine 324/5 mAb (5E11). Images were captured under identical settings. To dephosphorylate receptors, permeabilized cells were treated with calf intestinal alkaline phosphatase (E) or ${lambda}$ phosphatase (F) before immunostaining with 5E11. HA-CXCR4-YFP- and 5E11-labeled CXCR4 images were pseudocolored as green and red, respectively, and merged using ImageJ software. Yellow in merged images represents S324/5 phosphorylated CXCR4. DIC images of the cells are shown (right). Representative images of cells analyzed from three independent experiments are shown. Bars, 10 µm.

To investigate the time course of phosphorylation, we treatedcells with CXCL12 for 5, 15, and 30 min and then assessed thephosphorylation status of CXCR4 on serine residues 324 and 325.We observed very little phosphorylation at 5 min (Figure 9,A and B), which peaked at 15 min (Figure 9, C and D) of agonisttreatment, a time point at which CXCR4 is predominantly on thecell surface and which coincides with the time at which we observedan enhanced interaction between CXCR4 and AIP4 (Figure 2). Wedid not observe any immunostaining at 30 min after agonist treatment(Figure 9, E and F), at which point most of the receptor hadbeen internalized, suggesting that the serine residues 324 and325 are dephosphorylated once the receptor appears on endosomes.Therefore, these data indicate that CXCR4 is simultaneouslyphosphorylated at the plasma membrane on serine residues 324and 325 but is dephosphorylated before or upon internalizationof the receptor onto endosomes. Together, these data suggesta mechanism whereby phosphorylation of serine residues 324 and325 at the plasma membrane promotes recruitment of AIP4 directlyto CXCR4.

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Figure 9. Time course of CXCR4 phosphorylation. HEK293 cells transiently expressing HA-CXCR4-YFP were incubated with vehicle or CXCL12 for 5 (A and B), 15 (C and D), or 30 (E and F) min. Cells were fixed, permeabilized, and immunostained with 5E11. HA-CXCR4-YFP- and 5E11-stained receptor images were pseudocolored as green and red, respectively, and merged using ImageJ software. Yellow in merged images represents S324/5 phosphorylated CXCR4. DIC images of the cells are also shown (right). Shown are representative images of cells analyzed from three independent experiments. Bars, 10 µm.

We next set out to determine the role of phosphorylation ofserine residues 324 and 325 on the localization of AIP4 to theplasma membrane. To do this, we performed TIRF microscopy onHEK293 cells transiently coexpressing AIP4-CFP and wild-typeHA-CXCR4, S324/5A or the phosphomimetic mutant S324/5D. Afterserum starvation, cells were treated with or without CXCL12and time lapse images were collected in TIRF mode to allow usto only focus on events occurring at or near the cell surface(evanescent field <500 nm). Figure 10A shows a representativecell from each transfection condition before and after agoniststimulation. In cells expressing wild-type CXCR4, we observedseveral AIP4-CFP puncta before stimulation, but their numberincreased upon agonist treatment (Figure 10A). Comparison ofthe puncta density (puncta per square micrometer) on the plasmamembrane before and after agonist treatment revealed that agonisttreatment promoted a significant increase in puncta densityof AIP4-CFP ( $~$ 30%) in cells expressing wild-type CXCR4 (Figure 10B),suggesting that AIP4 is recruited to the plasma membrane uponagonist activation of CXCR4. Cells expressing S324/5A, however,showed markedly lower AIP4-CFP puncta density in the absenceof agonist compared with cells expressing wild-type receptor(Figures 10, A and B). In addition, agonist treatment failedto increase the puncta density, consistent with the idea thatserine residues 324 and 325 are required for binding and recruitmentof AIP4 to the receptor at the cell surface. In contrast, cellsexpressing the phosphomimetic mutant S324/5D without agonisttreatment showed a puncta density that was similar to that ofcells expressing wild-type receptor that were treated with agonist,suggesting that a negative charge imparted by aspartic acidresidues 324 and 325 leads to enhanced binding and recruitmentof AIP4 to the plasma membrane. Interestingly, puncta densitydid not change significantly after agonist treatment. Together,our data suggest that the agonist-dependent phosphorylationof serine residues 324 and 325 in the C-tail of CXCR4 is responsiblefor the recruitment of AIP4 to or in the vicinity of the plasmamembrane.

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Figure 10. AIP4 localizes to the plasma membrane upon activation of CXCR4. (A) Time-lapse images were acquired in TIRF mode for HEK293 cells transiently coexpressing AIP4-CFP and HA-CXCR4-WT, S324/5A, or S324/5D before and after treatment with 100 nM CXCL12 at $~$ 23°C. In total, 121 images were acquired over a period of 10 min. Shown are representative images of cells before and after treatment with agonist from each transfection. Puncta represent AIP4-CFP clusters at or near the cell surface attached to the glass support (depth of evanescent field <500 nm). (B) The graph represents the average density of AIP4-CFP puncta within the evanescent field. The average puncta density was calculated from 15 time-lapse images per cell before agonist treatment from a total of eight, nine, and 10 cells examined from CXCR4, S324/5A, and S324/5D transfected cells, respectively, from three independent experiments. The data collected after agonist treatment represent the maximal average puncta density observed from 15 continuous time-lapse images per cell. Data were analyzed by a two-way ANOVA (p < 0.01), followed by a paired t test with a Bonferroni correction revealing a significant increase in puncta density after agonist treatment in cells expressing wild-type CXCR4 (*p < 0.05). Bar, 7 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The posttranslational modification of GPCRs with ubiquitin isimportant for endocytic trafficking (Marchese et al., 2008

).Although several GPCRs are modified with ubiquitin, the identitiesof the ubiquitin ligases and the mechanisms that control recruitmentof the ubiquitination machinery to these receptors remain largelyunknown. We showed previously that CXCR4 is modified with ubiquitinby the E3 ligase AIP4, which functions as an endosomal sortingsignal to target CXCR4 to multivesicular bodies and its subsequentdegradation (Marchese and Benovic, 2001

; Marchese et al., 2003

).In this study, we have attempted to determine the mechanismby which AIP4 is targeted to CXCR4. Collectively, our data showthat agonist activation can promote a direct interaction betweenCXCR4 and AIP4. To our knowledge, this represents the firstdescription of a direct interaction between an E3 ubiquitinligase and an activated GPCR. Unlike the β₂AR, which requiresarrestin-3 for the recruitment of the E3 ligase Nedd4-1 to thereceptor (Shenoy et al., 2001

, 2008

), arrestins do not playa role in AIP4-mediated ubiquitination of CXCR4 (Bhandari etal., 2007

). Moreover, our studies reveal that the interactionoccurs between CXCR4 C-tail serines residues and the WW domainsof AIP4, suggesting a novel recognition motif for WW domainsthat to our knowledge has not been described previously in theliterature.

The novel AIP4 recognition sequence on CXCR4 includes C-tailserine residues 324 and 325. Using a custom phospho-specificantibody, we show that CXCR4 is simultaneously phosphorylatedon serine residues 324 and 325 at the plasma membrane. The timeof maximal phosphorylation ( $~$ 15 min) coincides with the timewhen AIP4 interacts with CXCR4 as assessed by coimmunoprecipitationand FRET analysis (Figure 2) and when we observe increased AIP4puncta density near the plasma membrane by TIRF microscopy (Figure 10).These data are consistent with a mechanism whereby agonist-mediatedphosphorylation of serine residues 324 and 325 promotes AIP4recruitment and binding to the receptor at the cell surfacefor subsequent ubiquitination and degradation of CXCR4. Interestingly,both serine residues 324 and 325 are part of a previously characterizedstretch of amino acids that mediates CXCR4 degradation (Marcheseand Benovic, 2001). We have shown previously that agonist-promoteddegradation of S324/5A is blocked; and here, we show that thisis because this receptor mutant is unable to interact with AIP4upon agonist stimulation and is not ubiquitinated. We establishthat AIP4 is targeted to CXCR4 at the plasma membrane via anovel interaction that involves phosphorylated C-tail serineresidues and the WW domains of AIP4. As GPCRs contain a numberof serine and threonine residues within their C-tail and arecommonly regulated by phosphorylation, WW domain mediated bindingmay represent a general mode of interaction with GPCRs, suggestingthat AIP4 and/or other Nedd4-family members may have a broadrole in regulating GPCRs.

In addition to the plasma membrane, we observed increased FRETintensity between CXCR4-YFP and AIP4-CFP in an intracellularlocation, which is not surprising because we have shown previouslythat CXCR4 and AIP4 colocalize on endosomes (Marchese et al.,2003). This interaction may also be mediated by phosphorylationof serine residues 324 and 325 as overall cellular FRET intensitybetween receptor and AIP4 was decreased in the S324/5A expressingcells (Figure 5). However, this intracellular interaction islikely not mediated via simultaneous phosphorylation of theseresidues because we did not detect intracellular CXCR4 thatwas simultaneously phosphorylated on S324 and S325 (Figures 8and 9), suggesting that CXCR4 is dephosphorylated before orafter it has internalized onto endosomes. It is important tonote that the phospho-serine CXCR4 antibody 5E11 only recognizessimultaneous phosphorylation of residues S324 and S325 and notindividually phosphorylated S324 or S325, as determined by confocalimmunofluorescence microscopy (Supplemental Figure S2). It maybe possible that phosphorylation of serine residue 324 or 325individually is sufficient to promote AIP4 binding as bindingof GST-WW-I-IV to the individual CXCR4 phosphomimetic mutants(S324D and S325D) was also enhanced, compared with the wild-typereceptor (Figure 10B). Therefore, AIP4 may interact with endosomalCXCR4 through phosphorylation of either serine residue 324 or325, but this remains to be explored.

The novel recognition sequence within CXCR4 was surprising giventhat WW domains are thought to bind to proline-based recognitionsequences and that the C-tail of CXCR4 does not contain prolineresidues. All four WW domains of AIP4 have been shown to bindto proline-rich PY motifs (Winberg et al., 2000; Otte et al.,2003; Ingham et al., 2005b). We report here that WW domainsI and II may also recognize nonproline-based sequences. We donot believe this is because WW domains I and II adopt a uniquestructure that would allow them to bind to nonproline-baseddomains, because structural studies reveal that at least forWW domain I of Itch (the AIP4 mouse orthologue) the structureis similar to other WW domains (Otte et al., 2003). The abilityof a WW domain to recognize multiple motifs is not unprecedentedbecause several WW domains have been shown to interact withmultiple recognition sequences (Ingham et al., 2005a). Althoughit is possible that other regions of AIP4 contribute to theinteraction, their role in binding is likely to be minimal giventhat GST-AIP4 ${Delta}$ WW showed almost no binding to CXCR4.

Our data also reveal several common elements between WW domainrecognition of proline-based motifs and of the novel CXCR4 recognitionsequence we have defined in this study. Typically, the secondconserved tryptophan residue in WW domains is important forproline-residue–based recognition (Zarrinpar and Lim,2000). Our data indicate that this residue in both WW domainsI and II is also important for CXCR4 recognition, although preciselyhow it participates in the interaction remains to be determined.In addition, we have identified two conserved amino acid residueslocated at the analogous position in WW domains I (Gln297) andII (Asn329) that are important for mediating the interactionwith CXCR4. Interestingly, these residues are located at theanalogous position to an arginine residue located in the WWdomain of Pin1 that has been shown to be directly involved inbinding to phospho-Ser-Pro motifs (Verdecia et al., 2000). Thepositively charged group of Arg17 in the Pin1 WW domain makescontact with the negative charge of the phosphorylated Ser residueof the p(Ser)-Pro motif (Verdecia et al., 2000). Although Gln297and Asn329 carry neutral side chains, it is possible that phosphorylatedserine residues 324 and 325 may interact with WW domains I andII through hydrogen bonding with the amide side chains of Gln297and Asn329, but this will require high resolution structuralanalysis to confirm. It is interesting to note that WW domainsIII and IV do not have a glutamine or an asparagine residueat the analogous position, which may explain why these WW domainsdo not bind to CXCR4, although they have been shown to bindto PY motifs (Winberg et al., 2000; Hu et al., 2004). Thereforeit is likely that this novel noncanonical WW domain mediatedinteraction that we report here may apply to only a subset ofWW domains. Interestingly, several WW domains from other Nedd4-likeE3s also contain an asparagine or an arginine residue at thiscritical position (see Figure 4B for an alignment), raisingthe possibility that these WW domains may bind to serine and/orthreonine residues found in a similar context to those presentin CXCR4. Regardless, we clearly establish the importance ofseveral AIP4 WW domain residues in mediating the interactionwith CXCR4.

In summary, we show here that AIP4 can interact directly withthe C-tail of CXCR4 via a novel WW domain recognition sequencethat does not contain proline residues. Our data reveal a modelwhereby agonist activation and phosphorylation of CXCR4 leadsto the recruitment of AIP4 to the receptor such that ubiquitinationof nearby lysine residues can occur thus enabling the receptorto be targeted for lysosomal degradation. To our knowledge,this study establishes for the first time a mechanism wherebya HECT domain E3 ligase can be directly targeted to an activatedGPCR. Whether this will emerge as a general mechanism by whichE3 ligases are targeted to GPCRs remains to be determined.

ACKNOWLEDGMENTS

We thank Dr. JoAnn Trejo (University of California, San Diego)for critical review of the manuscript, Dr. Karie Scrogin forhelp with statistical analysis, and Dr. Zhanjia Hou for helpwith the TIRF experiments. Work was supported by a ScientistDevelopment grant from the American Heart Association (to A.M.) and by National Institutes of Health grant GM-075159 (toA. M.). D. B. is supported by a predoctoral fellowship fromthe American Heart Association.

Footnotes

This was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E08-03-0308)on December 30, 2008.

Address correspondence to: Adriano Marchese (amarchese{at}lumc.edu)

Abbreviations used: AIP4, atrophin-interacting protein 4; FRET, fluorescence resonance energy transfer; GPCR, G protein-coupled receptor; GST, glutathione transferase; HECT, homologous to E6-AP carboxy terminus; TIRF, total internal reflection fluorescence.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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