Neurofilament-M Interacts with the D1 Dopamine Receptor to Regulate Cell Surface Expression and Desensitization

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The Journal of Neuroscience, July 15, 2002, 22(14):5920-5930

Neurofilament-M Interacts with the D₁ Dopamine Receptor to Regulate Cell Surface Expression and Desensitization
Ok-Jin Kim¹, Marjorie A. Ariano², Robert A. Lazzarini³, Michael S. Levine⁴, and David R. Sibley¹
¹ Molecular Neuropharmacology Section, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland 20892-1406, ² Department of Neuroscience, The Chicago Medical School, North Chicago, Illinois 60064, ³ Department of Biochemistry and Molecular Biology, Mount Sinai School of Medicine, New York, New York 10029, and ⁴ Mental Retardation Research Center, University of California, Los Angeles, California 90095

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We used the yeast two-hybrid assay to identify novel proteins that interact with the D₁ dopamine receptor. The third cytoplasmicloop (residues 217-273) of the rat D₁ receptor was used as baitto identify clones encoding interacting proteins from a rat braincDNA library. This identified two clones encoding the C terminusof rat neurofilament-M (NF-M) (residues 782-846). The NF-M clonedid not interact with the third cytoplasmic loops of the rat D₂,D₃, or D₄ receptors, but showed weak interaction with that ofthe D₅ receptor. Coexpression of full-length NF-M with the D₁receptor in HEK-293 cells resulted in >50% reduction of receptorbinding accompanied by a reduction in D₁ receptor-mediated cAMPaccumulation. NF-M had no effect on the expression of other dopaminereceptor subtypes. Using a D₁ receptor-green fluorescent proteinchimera and confocal fluorescence microscopy, we found that NF-Mreduced D₁ receptor expression at the cell surface and promotedaccumulation of the receptor in the cytosol. Interestingly, theD₁ receptors that were expressed at the cell surface in the presenceof NF-M were resistant to agonist-induced desensitization. Cellularcolocalization of NF-M and the D₁ receptor in the rat brain wasexamined by epifluorescence microscopy. These experiments showedthat ~50% of medium-sized striatal neurons expressed both proteins.Colocalization was also observed in pyramidal cells and interneuronswithin the frontal cortex. Similar immunohistochemical analysesusing NF-M-deficient mice showed decrements in D₁ receptor expressioncompared with control mice. These results suggest that NF-M interactswith the D₁ receptor in vivo and may modify its expression andregulation.

Key words: D₁ receptor; neurofilament-M; yeast two-hybrid; interaction; desensitization; colocalization

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The molecular actions of dopamine are mediated by five distinct receptor subtypes, some of which exist in different proteinisoforms attributable to alternative RNA splicing (Neve and Neve,1997). These receptors belong to the G-protein-coupled receptor(GPCR) superfamily and are divided into two major subgroups, D₁-likeand D₂-like, on the basis of their structure, pharmacology, andtransductional properties (Neve and Neve, 1997). The D₁-like subfamilyis composed of the D₁ and D₅ subtypes, both of which transducetheir signals by increasing intracellular cAMP levels. The D₂-likesubfamily consists of the D₂, D₃, and D₄ receptors, all of whichcan diminish cAMP production and regulate calcium and potassiumion channels. Abnormal expression or regulation of dopaminergicreceptors has been hypothesized to underlie neurological and endocrinedisorders, including Parkinson's disease, schizophrenia, Tourette'ssyndrome, dystonia, essential hypertension, and hyperprolactinemia(Neve and Neve, 1997).

The regional expression and distribution of each dopamine receptor subtype in the CNS has been well described (McVittie etal., 1991; Huang et al., 1992; Levey et al., 1993; Ariano andSibley, 1994; Smiley et al., 1994; Bergson et al., 1995; Arianoet al., 1997a,b; Muly et al., 1998). Overall, the D₁ receptoris the most abundant and widely distributed subtype, followedclosely by the D₂ receptor. The D₃, D₄, and D₅ receptors are notas widely distributed and are expressed at lower levels than thepredominant D₁ and D₂ subtypes. Recent investigations have indicatedthat many of the dopamine receptor subtypes exhibit discrete subcellularlocalizations. For instance, within cortical pyramidal cells,the D₁ receptor is expressed predominantly in dendritic spines,whereas the D₅ receptor is found primarily in dendritic shafts(Smiley et al., 1994; Bergson et al., 1995). Similarly, striatalD₂ receptors are more concentrated in spiny dendrites and spineheads than in the somata of the medium spiny neurons (Levey etal., 1993). Both the D₁ and D₂ receptors have also been localizedwithin axonal terminals, although typically not within the sameprojection pathway (Huang et al., 1992; Levey et al., 1993; Smileyet al., 1994). The mechanisms involved in transport, sorting,and targeting dopamine receptor subtypes to these discrete subcellularlocations are entirelyunknown.

Recent studies have begun to elucidate mechanisms for neurotransmitter receptor trafficking, membrane insertion, and anchoring,particularly for ligand-gated ion channels. Various proteins havebeen identified that may play a role in the aggregation and immobilizationof glutamate receptors, including a family of PDZ domain-containingproteins that are involved in the synaptic localization of NMDAreceptors (O'Brien et al., 1998; Kim and Huganir, 1999). Similarly,AMPA receptors are associated with proteins such as GRIP and PICK1that may direct their sorting and synaptic expression (Dong etal., 1999; Kim and Huganir, 1999; Xia et al., 1999). The majorityof these proteins have been identified through protein-proteininteraction screens such as the yeast two-hybrid assay. We, andothers, have begun to screen for dopamine receptor interactingproteins that may direct the transport, subcellular distribution,and anchoring of these receptor subtypes. Here we report thatneurofilament-M (NF-M) is an interacting protein for the D₁ dopaminereceptor. The interaction of this neuronal cytoskeletal proteinwith the D₁ receptor appears to regulate its cell surface expressionand its ability to be desensitized byagonists.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Plasmid construction and cDNA library screening. The yeast strain EGY48 was purchased from Display Systems Biotech (Vista,CA). The third cytoplasmic domain of the rat D₁ dopamine receptor(amino acids Ile²¹⁷-Thr²⁷³) was amplified by PCR using the sense primer 5'-GTATCTACAGGATTGCCCAGAAGC-3'containing a BamH1 site and the antisense primer 5'-GCGTCTTTAGAACTTTCGTCTCCC-3'containing an XhoI site. This amplified PCR product was subclonedin-frame into the BamH1 and XhoI sites of the yeast expressionvector pEG202, resulting in plasmid pEG202-D₁^3rd encoding the LexA-D₁^3rd fusion protein. The third cytoplasmic domains of the D_2L, D₃,D₄, and D₅ dopamine receptors were amplified by PCR using thesense primers 5'-TCAAAATCTACATCGTCCTCCGGAAG-3', 5'-CCAGGATCTACATAGTCCTGAGG-CAAA-3',5'-TGGGCCACTTTCCGTGGCTTGCGGCG-3', and 5'-GTATCTACCGCAT-TGCGCAGGTGCAG-3',respectively, all containing a BamH1 site, and the antisense primers5'-GACTCACCGAAAGAAGAGGAAGACGAC-3', 5'-CTGGGTGG-CCTTC-TTCTCTCGAAGTGG-3',5'-CTCATCGCCTTGCG-CTC-CCTTCCAGTG-3', and 5'-TTTGAAGACCTTGGTCTCCTTCTTGAT-3',respectively, all containing an XhoI site. The individual PCRproducts were subcloned in-frame into the BamH1 and XhoI sitesof the yeast expression vector pEG202 encoding the LexA fusionprotein. The yeast expression vectors containing the N terminalhalf and the C terminal of the third cytoplasmic domain of theD₅ receptor were generated using the sense primers 5'-GTATCTACCGCATTGCGCAGGTGCAG-3'and 5'-CGGAGTCGTGGAGCCTATGAA-3', respectively, containing a BamH1site, and the antisense primers 5'-GCAACTCTGAGCATGCTCAGC-3' and5'-TTTGAAGACCTTGGTCTCCTTCTTGAT-3', respectively, containing anXhoI site. A rat whole-brain cDNA library, subcloned into pJG4.5,was purchased from Origene Technologies (Rockville, MD). Two hybridtechniques (DupLex-A system) were performed as described (user'smanual from Origene Technologies). For screening the cDNA library,the bait vector pEG202-D₁^3rd was transformed into yeast strain EGY48 using a lithium acetateprotocol after transforming EGY48 with a LacZ reporter plasmid,pSH18-34. Transformation of EGY48 with both LacZ reporter plasmidand the bait plasmid confirmed that there was no interaction betweenLexA-D₁^3rd and reporter operator for inducing the expression of LacZ indicatingno blue color on X-gal media lacking histidine and uracil. Also,there was no induction of leucine in EGY48 with bait plasmid showingno growth on media lacking histidine, uracil, and leucine. TheEGY48 strains harboring the reporter plasmids and the bait plasmidswere transformed with the rat cDNA brain library, and the transformantsexpressing the bait and interacting prey proteins were selectedon medium lacking histidine, uracil, and tryptophan. The positiveclones (His+, Ura+, Trp+) were selected for further characterization.Plasmids from the selected clones were isolated using the YeastDNA isolation system (Bio101, Inc., Vista, CA) and amplified inEscherichia coli. DNA sequencing was performed by the NationalInstitute of Neurological Disorders and Stroke sequencing facilityusing automatedmethods.

In vitro binding assays. To generate a fusion protein encoding the D₁ third cytoplasmic domain (amino acids 217-273) and poly-histidine,the D₁ third cytoplasmic domain fragment (BamH1-XhoI) was subclonedinto plasmid pQE32 digested with restriction endonucleases BamH1and SalI. This plasmid was then transformed into XL1blue bacteria.Bacterial fusion protein production was induced by addition of1 mM isopropyl-1-thio- $beta$ -D-galactopyranoside for 4 hr at 37°C.Insoluble fusion proteins were purified using Ni²⁺-nitrilotriacetic acid-Agarose. The cDNA encoding NF-M (aminoacids 782-846) was excised from clone pJG4.5.clone N3 as an EcoR1fragment and subcloned into pGEX5X1. This plasmid, pGEX5X1.NF-M(782-846), was transformed into E. coli strain BL21 gold, allowingthe expression of NF-M as a glutathione S-transferase (GST) fusionprotein. Bacterial fusion protein production was induced by additionof 1 mM isopropyl-1-thio- $beta$ -D-galactopyranoside for 4 hr at 37°C.Insoluble fusion protein was purified using glutathione-Agarose.His-tagged fusion proteins were immobilized with Ni²⁺-nitrilotriacetic acid-Agarose overnight at 4°C in binding buffer(50 mM sodium phosphate, pH 7.4, 10% glycerol, 0.05% Triton X-100with protease inhibitor mixture), and non-bound proteins wereremoved by washing with binding buffer four times. GST-fusionprotein or GST protein alone was incubated with the immobilizedHis-tagged D₁^3rd in 400 µl of binding buffer for 2 hr at 4°C. Proteins bound tothe immobilized resin were collected by centrifugation, washedtwo times with 500 mM NaCl in binding buffer and two times withbinding buffer, eluted in 2× SDS sample buffer, and separatedby SDS-PAGE (14% acrylamide gel). Proteins were transferred topolyvinylidene difluoride (PVDF) membranes using semidry transblotter.PVDF membrane was incubated with anti-GST mouse monoclonal antibody(0.1 µg/ml) as primary antibody for 1 hr at room temperature andwashed four times with TBST (100 mM Tris, pH 7.4, 150 mM NaCl,0.1% Tween 20) before incubating with secondary antibody, anti-mouseantibody conjugated with horseradish peroxidase (1:10,000), for30 min at room temperature. Membranes were washed four times withTBST and developed using Super signal west pico chemiluminescentsubstrate (Pierce, Rockford,IL).

Cell culture and transfections. Human embryonic kidney (HEK)-293-tsa201 cells were cultured in DMEM supplemented with 10%fetal calf serum, 1 mM sodium pyruvate, 50 U/ml penicillin, 50µg/ml streptomycin, and 10 µg/ml gentamycin. Cells were grownat 37°C in 5% CO₂ and 90% humidity. The full-length rat D₁ receptorexpression plasmid was transfected with or without the rat full-lengthNF-M expression plasmid (gift from Dr. H. Pant, National Instituteof Neurological Disorders and Stroke/National Institutes of Health)into HEK-293-tsa201 cells using the calcium phosphate precipitationmethod (Invitrogen). Cells were seeded in 100 or 150 mm² plates, and transfection was performed when cells were ~50% confluent.DNA and 60 µl (30 µl for radioligand binding assays alone) of2 M CaCl₂ were mixed in H₂O in a total volume of 1000 µl and thenslowly mixed with HEPES buffered saline (HBS). The reaction mixturewas incubated at room temperature for 25 min and then evenly addedto the cell culture dish containing 20 ml of fresh media. After18 hr, the transfection media was replaced with fresh media, andthe cells were divided for radioligand and cAMP production assays.Cells were harvested the next day for theassays.

Radioligand binding assays. Cells were harvested by incubation with 5 mM EDTA in Earle's balanced salt solution (EBSS) andcollected by centrifugation at 300 × g for 10 min. The cells wereresuspended in lysis buffer (5 mM Tris, pH 7.4, 5 mM MgCl₂, at4°C) and disrupted using a Dounce homogenizer followed by centrifugationat 35,000 × g for 20 min. The resulting membrane pellet was resuspendedin binding buffer (50 mM Tris, pH 7.4). The membrane suspension(final protein concentration = 20-30 µg per tube) was then addedto assay tubes containing [³H]SCH-23390 in a final volume of 1.0 ml. (+)-Butaclamol was addedat the final concentration of 3 µM to determine nonspecific binding.The assay tubes were incubated at room temperature for 1.5 hr,and the reaction was terminated by rapid filtration through GF/Cfilters pretreated with 0.3% polyethyleneimine. Radioactivitybound to the filters was quantitated by liquid scintillation spectroscopyat a counting efficiency of 47%.

Determination of cAMP production. Transfected HEK-293-tsa201 cells were seeded into 24-well plates (~150,000 cells per well)and cultured for 1 d before the experiment. To assess desensitization,the cultures were first incubated in the absence or presence ofdopamine with 0.2 mM sodium metabisulfite and 5 µM (+/ $-$ )-propranolol(to block endogenous $beta$ -adrenergic receptors) and in HDMEM (20mM HEPES buffered DMEM, pH 7.4 at 37°C). Subsequently, the cellswere washed four times with 400 µl of EBSS (37°C) and furtherincubated with various concentrations of dopamine in a total volumeof 250 µl at 37°C for 15 min in the presence of 30 µM Ro-20-1724,0.2 mM sodium metabisulfite, and 5 µM (+/ $-$ )-propranolol. The reactionwas terminated by discarding the supernatant and adding 200 µlof 3% perchloric acid per well. After incubating on ice for 30min, 80 µl of 15% KHCO₃ was added to the wells, and the plateswere further incubated for 10 min. The plates were then centrifugedfor 10 min at 1300 × g, and 50 µl of the supernatant from eachwell was subsequently transferred to a 1.2 ml tube containing250 µl of reaction mixture (150 µl of Tris-EDTA buffer, 50 µlof cAMP binding protein, and 50 µl of [³H]cAMP). After incubation at 4°C overnight, 250 µl of charcoal-dextranmix (1%) was added to each tube followed by incubation at 4°Cfor 15 min and then centrifugation for 15 min at 1300 × g. Radioactivityin the supernatant from each tube was quantified by liquid scintillationspectroscopy at a counting efficiency of 47%. cAMP concentrationswere calculated using a standard curve according to the protocolof the assaykit.

Immunofluorescence histochemistry. Specific polyclonal antisera generated in rabbits against the D₁ and D₂ receptor subtypeshave been characterized extensively (McVittie et al., 1991; Arianoand Sibley, 1994; Levine et al., 1996). A mouse monoclonal antibodyagainst neurofilament-160 kDa (NF-M) was purchased from ZymedLaboratories (South San Francisco, CA). The NF-M-deficient micehave been described previously (Elder et al., 1998a,b). We usedNF-M-deficient mice that had been back-crossed into the C57BL/6strain for six generations and C57BL/6 wild-type mice for controls.Tissue sections were obtained from fresh, frozen rat or mousebrains and stained simultaneously for immunofluorescence histochemistryor singly for the D₂ receptor subtype. The antisera were dilutedin PBS, pH 7.2, applied together (dilutions: D₁, 1:200; NF-M,1:100; D₂, 1:200) to the slide-mounted, fresh-frozen sectionsand incubated overnight at 4°C in a humidified environment. Thenext day, unbound primary antisera were rinsed off, and secondary,fluorescently labeled antisera (donkey anti-rabbit or donkey anti-mouse,conjugated to either Cy2 or Cy3; Jackson ImmunoResearch, WestGrove, PA) were diluted 1:200 in PBS and applied for 2 hr at 4°Cin a humidified environment. Additional experiments examined individualimmunofluorescence detection of the D₁ receptor or NF-M to validatethat combined, simultaneous detection of the two proteins didnot compromise the respective individual expression patterns.Controls included using multiple D₁ receptor antisera, directedagainst different epitopes of the D₁ receptor protein sequence,and omission of the primary antisera. No differences were notedbetween double- or single-label immunofluorescenceincubations.

Fluorescence microscopy. Brain sections processed for immunohistochemistry were examined using standard epifluorescence microscopy(Olympus BX41). Digitized images of the experimental tissues indifferent brain areas were made with a megapixel camera (Optronics,Goleta, CA). Image acquisition parameters for each antisera stainingexperiment were optimized to use the entire grayscale range (0-255).At least four different experimental incubations were evaluatedfor the combined D₁ and NF-M staining. The fluorescent stainingreactions were stored and electronically merged using Adobe Photoshopoff-line.

Confocal microscopy. HEK293 cells were cultured in DMEM supplemented with 10% fetal calf serum, 1 mM sodium pyruvate, 50 U/mlpenicillin, 50 µg/ml streptomycin, and 10 µg/ml gentamycin. Cellswere grown at 37°C in 5% CO₂ and 90% humidity. Cells were seededon glass-bottom poly-D-lysine-coated 35 mm plates (MatTek Corporation,Ashland, MA) before the transfection with a D₁ receptor taggedwith GFP (D₁-GFP) or D₁-GFP and NF-M. Cells were washed with thefresh media the next day. Twenty-four to 36 hr after transfection,cells were subjected to confocal fluorescence microscopy(LSM410).

Data analysis. Radioligand binding assays were routinely performed in triplicate and repeated three to nine times. cAMP experimentswere performed in duplicate and repeated three to four times.Estimation of the radioligand binding parameters, K_D and B_max,as well as the EC₅₀ values for dopamine stimulation of cAMP production,were calculated using the GraphPad Prizm curve-fittingprogram.

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INTRODUCTION
MATERIALS AND METHODS
RESULTS
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REFERENCES

Interaction of NF-M with the third cytoplasmic loop of the D₁ dopamine receptor

To identify proteins that interact with the D₁ dopamine receptor, a yeast two-hybrid screen was performed using the thirdcytoplasmic loop (amino acids Ile²¹⁷-Thr²⁷³) of the D₁ receptor protein as bait (Fig. 1A). A total of 4 ×10⁶ library transformants were screened, resulting in the identificationof eight positive cDNA clones. These cDNAs were sequenced, andtwo identical clones encoding a C-terminal fragment of NF-M wereselected for further study. NF-M is a midsized intermediate filamentprotein with well defined head, helical rod, and C-terminal taildomains (Fig. 1B). In neurofilaments, the C-terminal tail domainsare greatly extended, relative to other intermediate filaments,and contain glutamic acid-rich regions of unknown significance(Lee and Cleveland, 1996; Elder et al., 1998a,b). Both of thepartial-length cDNAs encoded the last 65 residues of the NF-MC terminus (residues 782-846) as well as ~0.5 kb of 3' untranslatedsequence (Fig. 1B).

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Figure 1. Diagrams of rat D₁ dopamine receptor and NF-M proteins. A, Structure of the rat D₁ dopamine receptor as it is believed to be organized in the plasma membrane. Solid circles represent the portion of the third cytoplasmic loop (amino acids Ile²¹⁷-Thr²⁷³) that was used to construct the bait protein for the yeast two-hybrid screen. B, Diagram of the rat NF-M protein showing the head, helical rod, and tail regions of the 160 kDa protein. The region of the NF-M protein found to interact with the third cytoplasmic loop of the D₁ receptor is indicated at the C end of the tail domain.

To evaluate the specificity of the D₁ receptor-NF-M interaction, we examined the interaction of the partial-length NF-M clonewith the third cytoplasmic domains of all dopamine receptor subtypes(Table 1). No interaction was detected with any of the D₂ subfamilyof receptors, D_2L, D₃, or D₄; however, a very weak interactionwas detected with the third cytoplasmic loop of the D₅ receptor(Table 1). The D₁ and D₅ receptors show high sequence homology,especially within the putative transmembrane spanning domains(Fig. 2). The sequences are more divergent in intracellular domains;however, within the third cytoplasmic loops, the N-terminal regionsshow higher homologies compared with the C-terminal regions (Fig.2). We thus decided to test which area of the third cytoplasmicloop of the D₅ receptor weakly interacted with the NF-M clone.We prepared two bait plasmids, one consisting of the N-terminalarea of the third cytoplasmic loop of the D₅ receptor (residuesIle²²²-Cys²⁴⁵) and the other consisting of the C-terminal area of this loop(residues Arg²⁴⁶-Thr²⁷⁰) (Fig. 2). These bait plasmids were then evaluated using theyeast two-hybrid assay (Table 1). As shown, the N-terminal regionof the third cytoplasmic loop of the D₅ receptor interacted withthe NF-M clone; however, the C-terminal region did not. The interactionof the D₅ receptor N-terminal third loop fragment was not as strong,however, as the third cytoplasmic loop of the D₁ receptor (Table1).


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Table 1. Yeast two-hybrid interactions of the NF-M clone with the third cytoplasmic loops of all dopamine receptors

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Figure 2. Structure of the rat D₅ dopamine receptor. The black residues are identical between the D₁ and D₅ receptors. The line in the third cytoplasmic loop designates the end and the beginning of the N-terminal and C-terminal bait proteins, respectively (see Results).

These results suggest that the corresponding area of the D₁ receptor, the N-terminal region of the third cytoplasmic loop,is part of the NF-M interaction domain. To test this further,we prepared corresponding bait proteins consisting of the N-terminal(Ile²¹⁷-Cys²⁴¹) and C-terminal (Gln²⁴²-Thr²⁷³) fragments of the third cytoplasmic loop of the D₁ receptor andtested them using the two-hybrid assay (Table 1). Surprisingly,both of these fragments were positive with respect to interactingwith NF-M; however, when tested individually, their interactionswith NF-M were not as strong as that seen when the entire thirdcytoplasmic loop was used (Table 1). These results suggest thatNF-M actually interacts with multiple residues throughout theentire third cytoplasmicloop.

The specificity of the interaction of the NF-M clone with the third cytoplasmic loop of the D₁ receptor was further confirmedusing an in vitro binding assay (Fig. 3). For this experiment,we constructed a GST fusion protein with the NF-M clone and apolyhistidine-tagged construct of the third cytoplasmic loop ofthe D₁ receptor (D₁^3rd-His). Both of these proteins were expressed in bacteria and usedfor the in vitro binding assay. Figure 3 shows an SDS-PAGE gelblotted with antisera raised against the GST protein. Lanes 4and 5 show the NF-M-GST fusion protein and GST alone, respectively.Lanes 1-3 show eluates from a nickel gel to which the D₁^3rd-His protein was first adsorbed. Lane 1 shows D₁^3rd-His alone, lane 2 shows co-adsorbtion with the NF-M-GST fusionprotein followed by washing before elution, and lane 3 shows co-adsorbtionwith GST alone. Lane 6 shows NF-M-GST adsorption to the nickelgel in the absence of the D₁^3rd-His protein. The NF-M-GST protein is retained on the gel onlyin the presence of the D₁^3rd-His protein (lane 2), thus demonstrating a direct interactionbetween these proteins.

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Figure 3. In vitro binding assay. Bacterial fusion proteins, D₁^3rd-His and NF-M-GST, were produced as described in Materials and Methods. D₁^3rd-His was immobilized with Ni²⁺-nitrilotriacetic acid-Agarose overnight at 4°C (Lane 1-3). NF-M-GST (lane 2) or GST alone (lane 3) was next incubated with the immobilized D₁^3rd-His protein for 2 hr at 4°C. Lane 6 shows NF-M-GST incubated with the gel in the absence of D₁^3rd-His. Non-bound proteins were removed by washing. Proteins remaining bound to the immobilized resin were collected by centrifugation, washed, and eluted in SDS sample buffer. Lanes 4 and 5 show the NF-M-GST and GST proteins directly dissolved in SDS-PAGE sample buffer. Samples were subjected to SDS-PAGE and blotting as described in Materials and Methods. The experiment shown is representative of three such experiments.

Effect of NF-M on D₁ receptor expression in HEK293 cells

To investigate functional interactions between NF-M and the D₁ receptor, we coexpressed the proteins and examined the effecton receptor expression levels. Figure 4A shows the results ofoverexpressing the full-length rat NF-M protein on the expressionof the D₁ receptor in HEK293 cells. In the presence of NF-M, themaximum binding capacity of the D₁ receptor is reduced by >50%in the HEK293 cell membranes. This appears to be an effect onthe total receptor number in the membranes as opposed to a changein affinity for the radioligand (Fig. 4A). Because equal amountsof DNA were used in each transfection group, the decreased expressionof the D₁ receptor appears to be a direct result of NF-M expressionrather than a decreased efficiency of transfection for the D₁receptor construct.

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Figure 4. Effect of NF-M on D₁ and D₅ receptor expression. HEK293-tsa201 cells were transfected as described in Materials and Methods either with just the receptor expression plasmids (D₁/D₅ only) or with an expression vector encoding the full-length rat NF-M protein (D₁/D₅ + NF-M). Equal amounts of receptor expression vectors were added, and an appropriate amount of empty expression vector was included in the D₁/D₅ only groups such that equal amounts of DNA would be used in each transfection. Saturation radioligand binding assays in cell membranes using the D₁-like selective radiolabeled antagonist, [³H]SCH23390, were performed as described in Materials and Methods. A, The experiment shown for the D₁ receptor is representative of three such experiments. The binding parameters of this experiment are as follows: D₁ ONLY, K_d = 0.26 nM, B_max = 22 pmol/mg; D₁ + NF-M, K_d = 0.24 nM, B_max = 8.2 pmol/mg. B, The experiment shown for the D₅ receptor is representative of three such experiments. The binding parameters of this experiment are as follows: D₅ ONLY, K_d = 0.89 nM, B_max = 17 pmol/mg; D₅ + NF-M, K_d = 0.99 nM, B_max = 14 pmol/mg.

In contrast to the reduction in D₁ receptor expression by NF-M, there was no effect of coexpressing full-length NF-M on theexpression of the D₂ subfamily of receptors, D₂, D₃, or D₄ (datanot shown). These results are consistent with the yeast two-hybridresults shown in Table 1 and demonstrate that the effects ofNF-M on D₁ receptor expression are specific. Figure 4B shows theeffects of coexpressing NF-M on the expression of the D₅ receptor.In this case, the results were variable in that sometimes a smalldecrease in expression was observed, whereas in other experimentsthere was no effect. These observations are congruent, however,with the weak interaction that was observed with the partial-lengthNF-M clone and the third cytoplasmic loop of the D₅ receptor assessedusing the yeast two-hybrid assay (Table 1). Taken altogether,the results in Table 1 and Figure 4 indicate that NF-M specificallyinteracts with the D₁ receptor and that one consequence of thisinteraction is to diminish receptor binding activity in HEK293cells.

To further examine the effect of NF-M on D₁ receptor expression, we used a D₁ receptor construct in which the green fluorescentprotein (GFP) was fused to the C terminus of the receptor. Thisenables us to visualize the subcellular location of the D₁ receptorusing confocal fluorescence microscopy. Figure 5 shows the expressionof the D₁ receptor-GFP construct in HEK293 cells in the absenceand presence of NF-M. In the absence of NF-M, the receptor isexpressed predominantly in the plasma membrane at the cell surfacewith little internal fluorescence observed (Fig. 5, top panel).In contrast, in the presence of NF-M, a large fraction of theD₁ receptor appears to be located intracellularly, although someis still expressed at the cell surface (Fig. 5, bottom panel).Addition of dopamine to the cotransfected cells had no effecton these results (data not shown). The data in Figure 5 may providea morphological explanation for the experiment shown in Figure4A, which primarily assessed D₁ receptor binding in the plasmamembrane. Coexpression of NF-M in HEK293 cells apparently reducesthe cell surface expression of the D₁ receptor and concomitantlyincreases its intracellular accumulation.

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Figure 5. Expression of D₁ receptor-GFP in HEK293 cells. The subcellular distribution of the D₁ receptor-GFP in HEK293 cells was assessed using confocal fluorescence microscopy. The D₁ receptor-GFP construct was transfected with or without NF-M as described in Figure 4 using HEK293-tsa201 cells seeded on the bottoms of poly-D-lysine-coated glass plates. Thirty-six hours subsequent to transfection, the medium was changed to DMEM supplemented with 25 mM HEPES without phenol red before examining the cells using confocal fluorescence microscopy as described in Materials and Methods. Top panel shows D₁-GFP receptor expression in the absence of NF-M, whereas the bottom panel shows expression in the presence of NF-M. An experiment representative of three is shown.

Effect of NF-M on D₁ receptor function in HEK293 cells

We next examined the ability of the receptor to increase intracellular cAMP accumulation when stimulated by agonists to furtherinvestigate functional interactions between NF-M and the D₁ receptor.Figure 6A shows the effect of coexpressing the full-length NF-Mprotein on D₁ receptor activation of adenylyl cyclase and cAMPaccumulation in the HEK293 cells. In the absence of NF-M, dopaminestimulation of the D₁ receptor produces a robust and potent accumulationof cAMP in the HEK293 cells (Fig. 6A). In the presence of NF-M,the maximum response to dopamine is decreased by ~50%; however,the potency for dopamine is unaffected (Fig. 6A). Interestingly,the magnitude of the effect of NF-M on decreasing maximal receptor-mediatedcAMP accumulation is similar to that of decreasing the expressionof the receptor on the cell surface (Fig. 4A). This may suggestthat the decreased cAMP response is caused directly by the decreasedreceptor expression in the plasma membrane.

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Figure 6. Effect of NF-M on D₁ and D₅ receptor-stimulated cAMP accumulation. HEK-293-tsa201 cells were transfected with equal amounts of the D₁ or D₅ receptor expression constructs and with either the NF-M expression construct or an appropriate amount of empty vector. One day subsequent to the transfection, the cells were used for cAMP generation as described in Materials and Methods. A, The closed squares indicate HEK293-tsa201 cells transfected with the D₁ receptor alone, whereas the open squares indicate cotransfection with the D₁ receptor and NF-M. The data are expressed as a percentage of the maximal response in the absence of NF-M. An experiment representative of three is shown. In the experiment shown, the following EC₅₀ values were calculated: D₁ ONLY, EC₅₀ = 0.10 µM; D₁ + NF-M, EC₅₀ = 0.13 µM. B, The closed squares indicate HEK293-tsa201 cells transfected with the D₅ receptor alone, whereas the open squares indicate cotransfection with the D₅ receptor and NF-M. The data are expressed as a percentage of the maximal response in the absence of NF-M. An experiment representative of three is shown. In the experiment shown, the following EC₅₀ values were calculated: D₅ ONLY, EC₅₀ = 15 nM; D₅ + NF-M, EC₅₀ = 14 nM.

We also examined the effect of NF-M expression on the cAMP accumulation induced with the D₅ receptor. Figure 6B shows thatoverexpression of NF-M in the presence of the D₅ receptor producesminimal effects on receptor-stimulated cAMP accumulation in theHEK293 cells. These results are consistent with those shown inFigure 4B for D₅ receptor expression and further suggest thatNF-M interacts minimally, if at all, with the D₅ receptor in intactcells.

As a further approach to evaluate functional modification of D₁ receptor activity by NF-M, we examined agonist-induced desensitizationin the HEK293 cells. As with most G-protein-coupled receptors,the D₁ receptor undergoes functional desensitization when activatedwith agonists (for review, see Sibley and Neve, 1997). This responseappears to be mediated by receptor phosphorylation (Ng et al.,1994; Tiberi et al., 1996; Gardner et al., 2001) followed by associationwith $beta$ -arrestin (Zhang et al., 1999) and is manifested by reducedcAMP generation in response to agonists. D₁ receptor desensitizationhas been demonstrated previously using HEK293 cells (Tiberi etal., 1996). Figure 7 shows an experiment using HEK293 cells thatwere transfected with the D₁ receptor alone or when coexpressedwith NF-M. In the absence of NF-M, pretreatment of the cells withdopamine results in a diminished cAMP response when subsequentlyrechallenged with agonist (Fig. 7). In the presence of NF-M, thereis a reduced response to dopamine under basal conditions, as observedin the experiment shown in Figure 6A. Surprisingly, in the presenceof NF-M, pretreatment with dopamine had no further effect on D₁receptor activity (Fig. 7). Thus, coexpression with NF-M in theHEK293 cells appears to abolish desensitization of the D₁ receptorby agonists.

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Figure 7. Effect of NF-M on agonist-induced desensitization of the D₁ receptor. HEK-293-tsa201 cells were transfected with equal amounts of the D₁ receptor expression construct and with either the NF-M expression construct or an appropriate amount of empty vector as described in Figure 4. The cells were washed with EBSS and then incubated in media alone (controls) or in the presence of 10 µM dopamine for 30 min to induce desensitization as described in Materials and Methods. The cells were subsequently washed with EBSS and processed for the cAMP assays as described in Figure 6. The data are expressed as a percentage of the maximal response of the control group in the absence of NF-M. Closed squares represent D₁ receptor transfection only, without dopamine pretreatment; open squares represent the same transfection group with the dopamine pretreatment. Closed circles represent D₁ receptor and NF-M cotransfection without dopamine pretreatment; open circles represent the same transfection group with the dopamine pretreatment. This representative experiment was performed three times with similar results.

Cellular coincidence of NF-M and the D₁ receptor in the brain

We next assessed whether the interactions between NF-M and the D₁ receptor characterized in HEK293 cells might be meaningfulin the brain. We hypothesized that coexpression of the two proteinsmust occur to consider NF-M as a viable dopamine receptor-interactingprotein. Antisera directed toward the second extracellular loopof the rat D₁ receptor and a monoclonal antibody directed againstthe C-tail region of rat NF-M were used to examine the cellularexpression patterns of these proteins in various brain regions.The labeling for the D₁ receptor subtype in the striatum was visiblewithin a population of medium-sized neurons (~20 µm diameter)(Fig. 8A, arrows). Striatal neuropil, corresponding to dendriticprocesses, axon collaterals, and synaptic regions, also exhibitedD₁ receptor staining, as determined by the difference in fluorescentsignal visible in this tissue compartment contrasted with theunstained myelinated fibers of passage in the internal capsule.This distribution is analogous to our previous findings (Arianoand Sibley, 1994; Levine et al., 1996). NF-M was expressed throughoutthe striatal neuropil, in cell bodies (Fig. 8B, arrows), and insome axons within the internal capsule. These images were mergedelectronically to demonstrate the overlap of the Cy3 and Cy2 signalsused to detect the D₁ receptor and NF-M, respectively, in Figure8C. Areas of coexpression are visible as yellow-stained cell bodies(arrows) and processes within the neuropil. Some striatal neuronsexpressed only D₁ receptor (arrowheads) and appear as red-orangesomata. We estimate that approximately half of the striatal neuronscolocalize both proteins.

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Figure 8. Coexpression of D₁ receptor protein and NF-M in the rat striatum. Scale bar applies to all panels. A, D₁ protein was detected using an antisera directed against the second extracellular loop of the receptor. Staining is visible within the thin cytoplasmic rim of medium-sized neurons (arrows) and within the neuropil as a red (Cy3) reaction. Fiber bundles of the internal capsule do not show signal. B, NF-M was detected using a monoclonal antibody directed against a phosphate-independent epitope in the C-tail domain of the filament. The protein is expressed within neurons (arrows) and filaments throughout the striatum as bright green (Cy2) signals. Some axons coursing in the myelinated fibers within the internal capsule are seen. C, The D₁ and NF-M images were merged electronically to demonstrate coexpression of the proteins. Coincidence is detected as a yellow signal in >50% of the neurons (arrows) and also throughout the neuropil. Some neurons only express the D₁ receptor (arrowheads). This experiment was performed three times with similar results.

We also examined the distribution of the D₁ receptor and NF-M within rostral areas of the cortex overlying the striatum (Fig.9). A subgroup of layer 3 and layer 5 pyramidal neurons demonstratedcolocalization of both proteins (arrows), especially evident withintheir somata. Subcellular areas of overlap of the D₁ receptorand NF-M appear juxtaposed to the plasmalemma (Fig. 9B) and extenda short distance into the proximal portions of the apical andbasilar dendrites of labeled pyramidal neurons. Single-labeled,D₁ receptor-expressing pyramidal cells and interneurons are visiblethroughout the cortical laminations (arrowheads) and appear asred-orange somata. NF-M is localized prominently within the coreof the apical dendrites of pyramidal neurons (Fig. 9A) and withina fine network of fibrils visible at higher magnification in thecortical neuropil (Fig. 9B).

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Figure 9. Coexpression of D₁ receptor protein and NF-M in the rat somatosensory cortex. The pial surface is toward the top in each panel. A, Low-power image showing the coincident expression of the proteins as yellow signals (arrows) in the merged photomicrograph. Cell bodies expressing D₁ receptor only (arrowheads) are visible throughout the cortical laminae as red-stained elements. NF-M is readily detected within the apical dendrites of pyramidal cells in the more superficial layers of the cortex as a green signal. B, Higher magnification of layer 5 of the rat cortex demonstrates the colocalization of the D₁ receptor with NF-M in two pyramidal neurons (arrows). Single D₁-positive labeled somata (arrowheads) are visible, as well as neuronal processes that are positive for NF-M alone. This experiment was performed three times with similar results.

Dopamine receptor expression in NF-M-deficient mice

To further evaluate the effect of NF-M on D₁ receptor expression in the intact brain, we examined D₁ receptor staining inthe cortex and striatum of mice lacking NF-M. The NF-M-deficientmouse demonstrates diminished size in large and small diameteraxons in the central and peripheral nervous systems (Elder etal., 1998a,b). We also noted attenuation in the thickness of thecorpus callosum and a decrease in the diameter of the myelinatedfiber bundles of the internal capsule in the NF-M-deficient mouse(data not shown). There was a noticeable decrement in the levelof D₁ receptor subtype staining within the cortex and striatumof the NF-M-deficient mouse, and this is demonstrated for thefrontal cortex in Figure 10. The intensity of the fluorescent signalis decreased in the NF-M knock-out mouse compared with wild type,as shown in the lower-magnification images (Figs. 10A,B) whichspan the cortical laminations from layer 2 at the top edge ofthe image to layer 6 at the bottom edge of the photomicrograph.In addition, there are fewer D₁ receptor-positive cells in theNF-M-deficient mouse. Cortical cell counts revealed that therewere 47% fewer cells staining positive for the D₁ receptor inthe NF-M-deficient mouse. Moreover, cortical pyramidal neuronsin the NF-M-deficient mouse do not demonstrate proximal stainingin the apical dendrites for the D₁ receptor and seem to have lesspronounced pyramidal cytoarchitecture (Fig. 10, compare C, D).As a control for these results, we examined the immunofluorescentdistribution pattern of the D₂ receptor, which we have determineddoes not interact with NF-M. There were no qualitative or quantitativedifferences in the expression of the D₂ receptor in the NF-M-deficientmouse compared with wild-type tissue (Fig. 11).

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Figure 10. Cellular expression of the D₁ receptor in wild-type or NF-M-deficient mice is shown in the frontal cortex. The pial surface is toward the top edge of each image. Scale bar is the same for A-D. A, D₁ receptor staining in the wild-type (WT) is detected throughout the cortical laminas in somata and the neuropil. B, D₁ receptor staining is reduced substantially throughout the NF-M knock-out (KO) mouse cortex. C, D₁ receptor staining is detected within pyramidal and nonpyramidal neuron populations, as well as in the cortical neuropil in the WT. D, D₁ subtype staining is diminished in the KO, and the pyramidal neurons lack a prominent apically oriented cell body. This experiment was performed in two sets of wild-type and knock-out animals with similar results.

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Figure 11. Cellular expression of the D₂ receptor in wild-type or NF-M-deficient mice is shown in the frontal cortex. The pial surface is toward the top edge in each image. Scale bar applies to both photomicrographs. A, D₂ receptor expression is visible within the somata of pyramidal and nonpyramidal neurons of the wild-type (WT) mouse. The neuropil exhibits some reaction for the receptor, corresponding to distribution of the protein along processes and at synaptic structures. B, D₂ receptor staining in the NF-M knock-out (KO) mouse appears equivalent to the WT expression pattern. This experiment was performed in two sets of wild-type and knock-out animals with similar results.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we have identified NF-M as an interacting protein for the rat D₁ dopamine receptor. NF-M was shown to directlyinteract with the third cytoplasmic loop of this receptor, andyeast two-hybrid analyses were used to demonstrate the specificityof this association. No interaction was observed between NF-Mand the third cytoplasmic loops of the D₂ subfamily of dopaminereceptors, whereas a weak association was detected with the thirdcytoplasmic loop of the D₅ receptor. The third cytoplasmic loopof the D₁ receptor is known to be important for G_s-protein activation(Kozell et al., 1994), thus suggesting that NF-M may affect D₁receptor coupling among other functions (see below). The partial-lengthNF-M cDNA that was originally isolated encoded the C-terminal65 amino acids of this protein. Hitherto, no function has beenascribed to this area of NF-M, although it is known to be highlyacidic (Lee and Cleveland, 1996). Interestingly, there are multiple,positively charged residues within the third cytoplasmic loopof the D₁ receptor, suggesting a possible means of association.Future mutagenesis experiments using both NF-M and the D₁ receptorwill be required to delineate the exact residues required fortheirinteraction.

Coexpression of the full-length NF-M and D₁ receptor proteins also demonstrated functional interactions confirming the yeasttwo-hybrid data and in vitro binding assays using the proteinfragments. The effect of overexpressing NF-M was a reduction inD₁ receptor binding activity in the HEK293 cell membranes. Specificityfor this effect was observed in that overexpression of NF-M hadno effect on other dopamine receptor subtypes (or minimal effecton the D₅ receptor). Confocal fluorescence microscopy, using aD₁ receptor-GFP chimera, revealed that NF-M overexpression promotedan accumulation of receptor in intracellular compartments. Thismay explain the reduced cell surface-plasma membrane expressionof the D₁ receptor observed in the presence of NF-M. It is notclear whether NF-M retards receptor trafficking to the cell surface,perhaps by associating with newly synthesized receptor, or whetherthe presence of NF-M promotes enhanced or constitutive internalizationof the receptor once it is expressed at the cell surface. Furtherexperimentation will be required to distinguish between thesepossibilities. It should be noted that the effects of NF-M onD₁ receptor expression in neurons in vivo might be quite differentfrom those observed from overexpression in fibroblast-like cells.The existence of subcellular structures such as neurites and postsynapticdensities, to which NF-M may target D₁ receptor expression (seebelow), provides a level of complexity not easily mimicked incellculture.

Overexpression of NF-M also reduced the maximal stimulation of D₁ receptor-mediated cAMP accumulation. This could be a directresult of reduced receptor expression in the plasma membrane;however, other possibilities cannot be ruled out. For instance,as noted above, the third cytoplasmic loop of the D₁ receptoris involved in G_s coupling leading to adenylyl cyclase activation.Overexpression of NF-M might interfere with G_s coupling throughits association with the third cytoplasmic loop of the receptorand thus attenuate cAMP accumulation. Another possibility is thatNF-M may induce constitutive desensitization of the D₁ receptor.In this case, the receptor would be partially desensitized inthe absence of previous agonist activation (Pei et al., 1994).This would be consistent with the above suggestion of constitutivereceptor internalization; however, it would not explain why thereceptor was not desensitized further with agonist treatment.None of these potential mechanisms for the diminished functionalresponse of the D₁ receptor are mutuallyexclusive.

It was interesting to observe that overexpression of NF-M negated agonist-induced desensitization of the D₁ receptor. As notedabove, one possible explanation would be that the receptor isalready substantially desensitized, although further desensitizationafter agonist treatment might be expected. Instead, we favor thehypothesis that NF-M association with the receptor may negativelymodulate its phosphorylation by protein kinases and/or $beta$ -arrestinassociation with the phosphorylated receptor protein. This couldbe attributable to NF-M physically preventing the associationof these regulatory proteins with the D₁ receptor or by alteringthe receptor conformation so as to preclude the association withthese other proteins. Obviously, the presence and level of expressionof NF-M has the potential to alter D₁ receptor signaling. In neuronsthat coexpress both proteins, D₁ receptor activity might be modulatedby the close proximity of NF-M in the region of the D₁ receptor,thus modulating its expression, coupling, ordesensitization.

Neurofilament proteins are the major elements of the cytoskeleton in neurons and are abundant throughout the perikarya, axons,and dendrites (Lee and Cleveland, 1996). Neurofilaments are mosthighly concentrated in large myelinated axons, suggesting a potentialrole in regulating axonal transport. Thus, NF-M might also beinvolved in the axonal transport of the D₁ receptor to specificpresynaptic locations such as the terminals of the striatonigralprojection pathway (Huang et al., 1992; Levey et al., 1993; Smileyet al., 1994). Neurofilament expression in dendrites is more diffuseand less organized than in axons; however, neurofilaments havebeen shown to be associated with postsynaptic densities. Thissuggests that NF-M may also be involved in targeting the D₁ receptorto specific subcellular neuronal locations such as dendritic spines(Smiley et al., 1994; Bergson et al., 1995) and other postsynapticlocations. These functions are difficult to demonstrate usingtransfected cells in vitro and require in vivo experimentationfor theirelucidation.

To begin to address this issue, immunohistochemical analyses were used to determine that the D₁ receptor and NF-M were coexpressedin subsets of neurons within the striatum and frontal cortex ofadult rat brain, substantiating that the NF-M could interact withthe receptor in normal brain. The striatal colocalization is mostlikely associated with spiny projection neurons, because thisneuron population constitutes the majority of somata within thenucleus. An analogous distribution pattern was detected in thecortex, where only a subset of pyramidal neurons expressed bothproteins. The D₁ receptor staining did not extend into the distaldendrites of labeled cells, probably because of the level of resolutionthat we used. It is known that the D₁ receptor is trafficked inboth anterograde and retrograde directions to be distributed presynapticallyand postsynaptically (Smiley et al., 1994), but this necessitatesusing an electron microscopic study of the protein. The fact thatthere was not complete cellular overlap of NF-M and D₁ receptorstaining suggests that NF-M modulation of D₁ receptor functionmust be cell type-specific in theCNS.

To further substantiate in vivo interactions between NF-M and the D₁ receptor, we examined the cellular staining of the D₁receptor in brains from NF-M-deficient mice. D₁ receptor expressionin the striatum and cortex was decreased in these mice, in termsof both total positive cells and the intensity and distributionof staining. Notably, there appeared to be decreased stainingfor the D₁ receptor in the apical dendrites of the cortical pyramidalneurons. This may indeed suggest that NF-M assists in the targetingof the D₁ receptor to these neuronal structures. These resultsfurther suggest that it will be important to examine the NF-M-deficientmouse for alterations in D₁ receptor-mediatedbehaviors.

Recently, Huganir and colleagues (Ehlers et al., 1998) have used the yeast two-hybrid system to identify another intermediatefilament protein, neurofilament-L (NF-L), as an interacting proteinfor the NR1 NMDA receptor subunit. NF-L was shown to interactwith the NR1 subunit in a splice variant-specific manner and wasspeculated to be involved in anchoring or localizing NMDA receptorsin the neuronal plasma membrane, although specific effects onreceptor function were not demonstrated. NF-L thus appears tobelong to a family of cytoskeletal and scaffolding proteins thatare involved in targeting ligand-gated ion channels to synapticlocations (Kim and Huganir, 1999). Our data extend these findingsand describe the first direct interaction of a neurofilament proteinwith a GPCR. Neurofilament-GPCR interactions may be widespread,however, because activation of the angiotensin AT₂ receptor downregulatesNF-M expression in PC12W cells (Gallinat et al., 1997), and opiatetreatments of rats have been shown to increase neurofilament-Hphosphorylation in the brain (Jaquet et al., 2001).

Our results indicate that NF-M can be added to a growing list of proteins referred as DRIPs (dopamine receptor interactingproteins) that have been identified through various protein interactionscreens. Many of these proteins are structural or cytoskeletalelements. For instance, the actin binding protein filamin A (ABP-280)was found to modulate the cell surface expression of D₂ and D₃receptor subtypes (Bermak et al., 2001; Li et al., 2001). Anotheractin binding protein, spinophilin, has also been shown to directlyassociate with the D₂ dopamine receptor (Smith et al., 1999).Furthermore, a novel protein named DRiP78 has been identifiedthat regulates D₁ receptor transport from the endoplasmic reticulum(Bermak et al., 2001). Interestingly, overexpression of DRiP78retards the cell surface expression of the D₁ receptor. Furtherelucidation of the specific functions of these and other dopaminereceptor interacting proteins will greatly aid our understandingof dopamine receptor signaling and itsregulation.

  FOOTNOTES

Received Jan. 23, 2002; revised April 22, 2002; accepted April 29, 2002.

We thank Dr. H. Pant for providing the full-length NF-M cDNA, and Lindsey Christian and Ehud Gruen for technical assistance.This work was partially supported by Department of Defense Grant17-99-1-9542 to M.A.A. and National Institutes of Health GrantNS33538 to M.S.L.

Correspondence should be addressed to Dr. David R. Sibley, Molecular Neuropharmacology Section, National Institute of NeurologicalDisorders and Stroke/National Institutes of Health, Building 10,Room 5C108, 10 Center Drive, MSC 1406, Bethesda, MD 20892-1406.E-mail: sibley{at}helix.nih.gov.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ariano MA, Sibley DR (1994) Dopamine receptor distribution in the rat CNS: elucidation using anti-peptide antisera directed against D_1A and D₃ subtypes. Brain Res 649:95-110[ISI][Medline].
Ariano MA, Wang J, Noblett KL, Larson ER, Sibley DR (1997a) Cellular distribution of the rat D_1B receptor in CNS using anti-receptor antisera. Brain Res 746:141-150[ISI][Medline].
Ariano MA, Wang J, Noblett KL, Larson ER, Sibley DR (1997b) Cellular distribution of the rat D₄ dopamine receptor protein in the CNS using anti-receptor antisera. Brain Res 752:26-34[ISI][Medline].
Bergson C, Mrzljak L, Smiley JF, Pappy M, Levenson R, Goldman-Rakic PS (1995) Regional, cellular and subcellular variations in the distribution of D₁ and D₅ dopamine receptors in primate brain. J Neurosci 15:7821-7836[Abstract].
Bermak JC, Li M, Bullock C, Zhou Q-Y (2001) Regulation of transport of the dopamine D₁ receptor by a new membrane-associated ER protein. Nat Cell Biol 3:492-498[ISI][Medline].
Dong H, Zhang P, Song I, Petralia RS, Liao D, Huganir RL (1999) Characterization of the glutamate receptor interacting proteins GRIP1 and GRIP2. J Neurosci 19:6930-6941[Abstract/Free Full Text].
Ehlers MD, Fung ET, O'Brien RJ, Huganir RL (1998) Splice variant-specific interaction of the NMDA receptor subunit NR1 with neuronal intermediate filaments. J Neurosci 18:720-730[Abstract/Free Full Text].
Elder GA, Friedrich VL, Bosco P, Kang C, Gourov A, Tu PH, Lee VMY, Lazzarini RA (1998a) Absence of the mid-sized neurofilament subunit decreases axonal calibers, levels of light neurofilament (NF-L), and neurofilament content. J Cell Biol 141:727-739[Abstract/Free Full Text].
Elder GA, Friedrich VL, Margita A, Lazzarini RA (1998b) Age related atrophy of motor neurons deficient in the mid-sized neurofilamnet subunit. J Cell Biol 146:181-192.
Gallinat S, Csikos T, Meffert S, Herdegen T, Stoll M, Unger T (1997) The angiotensin AT₂ receptor down regulates neurofilament M in PC12W cells. Neurosci Lett 227:29-32[ISI][Medline].
Gardner B, Liu ZF, Jiang D, Sibley DR (2001) The role of phosphorylation/dephosphorylation in agonist-induced desensitization of D₁ dopamine receptor function: evidence for a novel pathway for receptor de-phosphorylation. Mol Pharmacol 59:310-321[Abstract/Free Full Text].
Huang Q, Zhou D, Chase K, Gusella JF, Aronin N (1992) Immunohistochemical localization of the D₁ dopamine receptor in rat brain reveals its axonal transport, pre- and postsynaptic localization, and prevalence in the basal ganglia, limbic system, and thalamic reticular nucleus. Proc Natl Acad Sci USA 89:11988-11992[Abstract/Free Full Text].
Jaquet PE, Ferrer-Alcon M, Ventayol P, Guimon J, Garcia-Sevilla JA (2001) Acute and chronic effects of morphine and naloxone on the phosphorylation of neurofilament-H proteins in the rat brain. Neurosci Lett 304:37-40[Medline].
Kim JH, Huganir RL (1999) Organization and regulation of proteins at synapses. Curr Opin Cell Biol 11:248-254[ISI][Medline].
Kozell LB, Machida CA, Neve RL, Neve KA (1994) Chimeric D₁/D₂ dopamine receptors. J Biol Chem 269:30299-30306[Abstract/Free Full Text].
Lee MK, Cleveland DW (1996) Neuronal intermediate filaments. Annu Rev Neurosci 19:187-217[ISI][Medline].
Levey AI, Hersch SM, Rye DB, Sunahara RK, Niznik HB, Kitt CA, Price DL, Maggio R, Brann MR, Ciliax BJ (1993) Localization of D₁ and D₂ dopamine receptors in brain with subtype-specific antibodies. Proc Natl Acad Sci USA 90:8861-8865[Abstract/Free Full Text].
Levine MS, Altemus KL, Cepeda C, Cromwell HC, Crawford C, Ariano MA, Drago J, Sibley DR, Westphal H (1996) Modulatory actions of dopamine on N-methyl-D-aspartate receptor-mediated responses are altered in D_1A-deficient mice. J Neurosci 16:5870-5882[Abstract/Free Full Text].
Li M, Bermak JC, Wang ZW, Zhou QY (2000) Modulation of dopamine D₂ receptor signalling by actin-binding protein (ABP-280). Mol Pharmacol 57:446-452[Abstract/Free Full Text].
Lin R, Karpa K, Kabbani N, Goldman-Rakic P, Levenson R (2001) Dopamine D₂ and D₃ receptors are linked to the actin cytoskeleton via interaction with filamin A. Proc Natl Acad Sci USA 98:5258-5263[Abstract/Free Full Text].
McVittie LD, Ariano MA, Sibley DR (1991) Characterization of anti-peptide antibodies for the localization of D₂ dopamine receptors in rat striatum. Proc Natl Acad Sci USA 88:1441-1445[Abstract/Free Full Text].
Muly III EC, Szigeti K, Goldman-Rakic PS (1998) D₁ receptor in interneurons of Macaque prefrontal cortex: distribution and subcellular localization. J Neurosci 18:10553-10565[Abstract/Free Full Text].
Neve KA, Neve RL (1997) In: The dopamine receptors. Totowa, NJ: Humana.
Ng GYK, Mouillac B, George SR, Caron M, Dennis M, Bouvier M, O'Dowd BF (1994) Desensitization, phosphorylation and palmitoylation of the human dopamine D₁ receptor. Eur J Pharmacol 267:7-19[ISI][Medline].
O'Brien RJ, Lau LF, Huganir RL (1998) Molecular mechanisms of glutamate receptor clustering at excitatory synapses. Curr Opin Neurobiol 8:364-369[ISI][Medline].
Pei G, Samama P, Lohse M, Wang M, Codina J, Lefkowitz RJ (1994) A constitutively active mutant $beta$ ₂-adrenergic receptor is constitutively desensitized and phosphorylated. Proc Natl Acad Sci USA 91:2699-2702[Abstract/Free Full Text].
Sibley DR, Neve KA (1997) In: Regulation of dopamine receptor function and expression in the dopamine receptors (Neve KA, Neve RL, eds), pp 383-424. Totowa, NJ: Humana.
Smiley JF, Levey AI, Ciliax BJ, Goldman-Rakic PS (1994) D₁ dopamine receptor immunoreactivity in human and monkey cerebral cortex: predominant and extrasynaptic localization in dendritic spines. Proc Natl Acad Sci USA 91:5720-5724[Abstract/Free Full Text].
Smith FD, Oxford GS, Milgram SL (1999) Association of the D₂ dopamine receptor third cytoplasmic loop with spinophilin, a protein phosphatase-1-interacting protein. J Biol Chem 274:19894-19900[Abstract/Free Full Text].
Tiberi M, Nash SR, Bertrand L, Lefkowitz RJ, Caron MG (1996) Differential regulation of the dopamine D_1A receptor responsiveness by various G protein-coupled receptor kinases. J Biol Chem 271:3771-3778