N‐glycosylation and expression in human tissues of the orphan GPR61 receptor

A number of members of the G protein‐coupled receptor class of cell surface receptors are ‘orphans’ with no known endogenous ligand. One of these orphan receptors is GPR61; there are little data about its expression in human cells and tissues. In this study, we investigated the post‐translational modification of GPR61 by N‐glycosylation at an identified consensus N‐glycosylation site (N12) and the impact of this modification upon the subcellular expression of the protein. The N‐glycosylation inhibitor tunicamycin reduced the apparent molecular weight of immunoreactivity associated with myc‐tagged GPR61 by 1–2 kDa, which was comparable to the evident molecular weight of the myc‐tagged N12S GPR61 mutant with disrupted consensus N‐glycosylation site. Analysis of GPR61 expression demonstrated that tunicamycin treatment reduced considerably heterologous expression of GPR61 in the cell membrane despite the N12S GPR61 mutant being readily expressed at the cell surface. These results demonstrate that GPR61 is subject to N‐glycosylation but suggest this is not a prerequisite for cell surface expression, although N‐glycosylation of other proteins may be important for cell membrane expression of GPR61. Expression of GPR61 protein was demonstrated at the cellular level in human hippocampus and human peripheral blood mononuclear cells. In the latter, there was a significantly higher expression of GPR61 in the Th17 cell subset in comparison with resting CD4+ cells, which may point toward a potential role for the GPR61 receptor in autoimmune diseases. This is the first report that GPR61 protein is subject to post‐translational modification and is expressed in immune cell subsets and the hippocampus. These findings will help guide studies to investigate the function of GPR61.

A number of members of the G protein-coupled receptor class of cell surface receptors are 'orphans' with no known endogenous ligand. One of these orphan receptors is GPR61; there are little data about its expression in human cells and tissues. In this study, we investigated the post-translational modification of GPR61 by N-glycosylation at an identified consensus N-glycosylation site (N12) and the impact of this modification upon the subcellular expression of the protein. The N-glycosylation inhibitor tunicamycin reduced the apparent molecular weight of immunoreactivity associated with myc-tagged GPR61 by 1-2 kDa, which was comparable to the evident molecular weight of the myc-tagged N12S GPR61 mutant with disrupted consensus N-glycosylation site. Analysis of GPR61 expression demonstrated that tunicamycin treatment reduced considerably heterologous expression of GPR61 in the cell membrane despite the N12S GPR61 mutant being readily expressed at the cell surface. These results demonstrate that GPR61 is subject to N-glycosylation but suggest this is not a prerequisite for cell surface expression, although N-glycosylation of other proteins may be important for cell membrane expression of GPR61. Expression of GPR61 protein was demonstrated at the cellular level in human hippocampus and human peripheral blood mononuclear cells. In the latter, there was a significantly higher expression of GPR61 in the Th17 cell subset in comparison with resting CD4+ cells, which may point toward a potential role for the GPR61 receptor in autoimmune diseases. This is the first report that GPR61 protein is subject to post-translational modification and is expressed in immune cell subsets and the hippocampus. These findings will help guide studies to investigate the function of GPR61.
G protein-coupled receptors (GPCRs) are the largest family of cell surface receptors and are the therapeutic targets for nearly a third of clinically marketed drugs [1], yet a number of human GPCRs remain poorly understood including lack of knowledge of their endogenous orthosteric ligand. Included in these so-called orphan receptors is GPR61 (other names: GPCR3, biogenic amine receptor-like G protein-coupled receptor, BALGR), which is predicted to be a 49-kDa GPCR that belongs to orphan receptors class A [2,3].
The quaternary structure and function of this receptor have not been revealed. The initial report identifying the GPR61 clone indicated that the amino acid sequence of GPR61 shares some degree of sequence similarity (28-31%) with certain histamine, adrenergic, serotonin, and dopamine receptors [2], although it was later suggested that GPR61 might be better grouped with melatonin receptors by phylogenetic clustering [4]. GPR61 mRNA is expressed across a wide range of tissues with brain, testis, and leukocytes having the highest apparent levels of expression [2,5]. Of relevance, recent immunohistochemistry (IHC) staining revealed that the zona glomerulosa has the highest expression of GPR61 within the human adrenal gland, with a potential link to aldosterone synthesis [6].
The first study reporting a potential low-affinity inverse agonist for GPR61 was published in 2003 [7]; 5-(nonyloxy)-tryptamine (5-NOT) impacted a chimeric receptor with high micromolar potency. Interestingly, there is some evidence for autoregulation of the receptor activity [8], its constitutive activity [9], although one previous work was not supportive [10].
Knowledge about cellular and physiological functions for GPR61 is inferred from studies with GPR61-knockout (ko) mice. These mice display elevated levels of liver triacylglycerols, plasma leptin, and insulin [11], which may underlie the greater fat mass and correlate with lower levels of hypothalamic proopiomelanocortin and brain-derived neurotropic factor mRNA. Such findings forward the GPR61 receptor as a target to regulate body weight and food intake and hence may provide a target for antiobesity drugs. In addition, GPR61 has also been proposed to play a role in aldosterone production [12].
Given the potential of the GPR61 receptor as a drug target for therapeutic benefit, we have studied the potential importance of N-glycosylation of GPR61 proteinthe functions of many GPCRs are influenced by this post-translational modification [13,14] and also investigated the presence of the protein in some human tissues.

Antibodies to GPR61
Specificity of commercially available anti-GPR61 antibody (sc-54599, SCT) was tested in flow cytometry and western blot using recombinant HEK293 cells, and it was confirmed that this antibody cannot be used to effectively assay for GPR61 expression in these cells. GPR61 antisera were provided by A. Davenport, and it was shown that GPR61transfected cells have significantly higher staining levels in flow cytometry than untransfected cells.

SDS/PAGE and western blotting
Cells were scraped off the culture flask and sonicated over wet ice. Following the sonication, samples were resuspended in an equal volume of 29 radioimmunoprecipitation assay buffer (RIPA; Cell Signaling Technology, Danvers, MA, USA) and appropriate volume of 29 urea sample buffer. No more than 30 lg of protein was loaded and run on 4-20% Tris/glycine gels (Bio-Rad, Hercules, CA, USA, cat. 4561094). For each gel, at least one molecular weight ladder was included (New England Biolabs, Ipswich, MA, USA, cat. P7712). Proteins were transferred onto PVDF membranes, which were then blocked in 10% nonfat milk (Marvel) for 2 h at room temperature. Membranes were incubated in 1 : 3000 anti-myc (Cell Signaling Technology) or 1 : 3000 anti-GAPDH (Abcam, Cambridge, UK) in 5% nonfat milk overnight at 4°C before washing at room temperature. Membranes were incubated subsequently in anti-mouse or anti-rabbit HRP-linked secondary antibody (Cell Signaling Technology) in 5% nonfat milk in wash buffer at room temperature for 2 h. Membranes were washed and then incubated in ECL reagent for 5 min. The membrane was subsequently exposed to film and developed. Alternatively, the membrane was developed using Che-miDoc MP system imager (Bio-Rad) that also allows for the subsequent quantification of chemiluminescent bands. Images acquired using ChemiDoc MP were analyzed in IMAGE LAB 5.2.1 software (Bio-Rad).

Immunocytochemistry
Cells were seeded at a density of 50 000 cells on poly-D-lysinecoated coverslips and cultured for 18 h at 37°C. The cells were then washed in PBS and fixed with 2% formaldehyde solution (Sigma Aldrich, St Louis, MO, USA, cat. F8775) for 15 min at room temperature and protected from light. After washing, for staining intracellular proteins, cells were permeabilized with 0.3% Triton X-100 (Sigma Aldrich, cat. X100) in PBS for 20 min at room temperature. The cells were then washed with PBS and blocked in 10% FBS in PBS (blocking buffer) for 1 h. After the blocking step, primary antibody solution (1 : 3000 anti-myc or 1 : 2000 GPR61 antisera) in blocking buffer was added and incubated overnight at 4°C. On the following day, primary antibody was removed by washing with PBS. Secondary antibody solution (1 : 1000 fluorochrome-conjugated secondary antibody; Thermo Fisher Scientific) in blocking buffer was then added and incubated for 3 h at room temperature. Cells were then washed in PBS.
In the experiments in which myc-tagged GPR61 was used to stain extracellularly and intracellularly, cells were permeabilized on the second day after the first application of the secondary antibody. The procedure was then repeated: Cells were incubated overnight at 4°C in a primary antibody solution. On the following day, the cells were washed and a different secondary antibody conjugated to a different fluorochrome at the same concentration was added in blocking buffer and left to incubate for 3 h at room temperature. After the incubation with the secondary antibody solution, the cells were washed with PBS. The coverslips containing the cells were then mounted on microscope slides with Vecta-Shield Hardset mounting medium containing DAPI (Vector Laboratories, Burlingame, CA, USA, cat. H-1500). Images were captured on the same day using Zeiss LSM Meta 510 confocal microscope and analyzed in LSM IMAGE BROWSER software (Zeiss, Oberkochen, Germany).
Myc immunoreactivity by flow cytometry HEK293 cells stably expressing His-myc-tagged GPR61 and untransfected HEK293 cells were used. Some cells were treated with 1.0 lgÁmL À1 tunicamycin (Sigma Aldrich) for 48 h to inhibit the N-glycosylation. Following the treatment, medium was aspirated from the cells and the cells were washed in PBS. The cells were then detached from the flask by the addition of 1 mM EDTA PBS and were left at 4°C for 10 min. The cells were transferred to complete DMEM and centrifuged twice at 400 g for 5 min. The supernatant was discarded and the cells were resuspended in 0.5% BSA/PBS. The cells were resuspended in 1 : 500 mouse anti-myc antibody in 0.5% BSA/PBS and incubated for 1 h at 4°C. The cells were then washed twice by centrifugation and resuspended in 1 : 200 goat antimouse PE (Abcam) in 0.5% BSA in PBS. The cells were incubated for 30 min at room temperature. The cells were then washed twice by centrifugation before resuspension in 0.5% BSA/PBS and immediately assayed using ADP Cyan flow cytometer (Beckman Coulter, Brea, CA, USA).

Hippocampus tissue samples and immunohistochemistry
Human formalin-fixed, paraffin-embedded hippocampal samples were obtained from the Medical Research Council, Edinburgh Brain and Tissue Bank (University of Edinburgh, Edinburgh, UK). The donors (aged 20-40, postmortem index 36-77 h) were free from neurological or psychological conditions. The study was approved by the University of Birmingham Ethics Committee.
The immunohistochemistry staining was conducted as previously described by Brady et al. [15].

Isolation of human peripheral blood mononuclear cells
Peripheral blood mononuclear cells (PBMCs) were isolated from whole blood from healthy donors or from leukocyte reduced system (LRS) cones using Ficoll-Paque (GE Healthcare, Little Chalfont, UK). In some experiments, cells were stimulated in the presence of PHA-L (5 lgÁmL À1 ; Roche, Basel, Switzerland) for 24 h.

RNA isolation from human hippocampus and PBMCs
Total RNA was isolated from human PBMCs using QIA-GEN RNeasy Mini Kit according to the manufacturer's instructions with DNase treatment included. RNA concentration and purity were measured on NanoDrop 2000, and RNA was stored at À80°C prior to the experiments.

GPR61 expression by PBMCs assessed by flow cytometry
PBMCs were stained with a panel of antibodies specific for cell surface markers (mouse anti-human CD4, CD8, CD14, and CD19; eBioscience, San Diego, CA, USA) for 20 min at 4°C in 10% FcR blocker (Miltenyi, Bergish Gladbach, Germany). The cells were then washed twice, fixed in Cytofix/Cytoperm (BD) for 15 min at 4°C, and permeabilized by washing in Perm buffer (Becton Dickinson, Franklin Lakes, NJ, USA) before being stained with GPR61 antisera or control preimmune sera for 30 min at 4°C. The cells were then washed twice and stained with AlexaFluor647-conjugated anti-goat antibody (1 : 2000; Thermo Fisher Scientific). The cells were washed twice and assayed on ADP Cyan flow cytometer.
For the assessment of GPR61 expression in IFN-c+ and IL-17+ cells, PBMCs were stimulated for 24 h with 5 lgÁmL À1 phytohemagglutinin-M at 37°C. After 24 h, the plate was centrifuged and the cells were restimulated with 50 ngÁmL À1 phorbol 12-myristate-13-acetate and  The consensus N-glycosylation sequence at N12 was disrupted by mutagenesis (N12S) with the arising myc-immunoreactive species displaying a lower apparent molecular weight compared with the nonmutated protein, and furthermore, the N12S mutant apparent molecular weight was unaffected by tunicamycin treatment. Data presented are from a single representative experiment, which was repeated at least five times with similar results. GAPDH was used as a loading control. 750 ngÁmL À1 ionomycin in the presence of 0.5 lL per well GolgiStop for 3 h at 37°C. After 3 h, the cells were washed twice by centrifugation. Cells were stained for surface markers as above. Cells were then fixed and incubated for 15 min at 4°C in the dark. The cells were then centrifuged twice in 19 Perm/Wash buffer. The cells were stained with anti-GPR61, anti-IFN-c, and anti-IL-17 antibodies for 20 min at 4°C. The cells were centrifuged twice and stained with the AlexaFluor647-conjugated anti-goat antibody. The cells were washed twice and assayed on ADP Cyan flow cytometer.

Statistical analysis
Statistical analysis was performed using PRISM 6 (Graph-Pad, La Jolla, CA, USA).

SDS/PAGE/western blotting
SDS/PAGE separation of lysates of HEK293 stably expressing nonmutated and N12S mutant myc-tagged . Subsequent permeabilization of cells followed by re-immunolabeling allowed visualization of myc-immunoreactive protein expressed throughout the cell (green immunofluorescence). DAPI stain (blue fluorescence) was used to visualize the cell nuclei. When the cell images were combined, immunoreactive protein expressed in the cell membrane appears yellow, whereas intracellular immunoreactive protein appears green. Treatment of cells with tunicamycin (1.0 lgÁmL À1 , 48 h) resulted in the reduced level of cell membrane myc immunoreactivity shown as reduced levels of red staining. Lower panel: The same as in the upper panel but the intracellular staining following the permeabilization was performed using anti-GPR61 sera and the resulting immunoreactivity appears green. The scale bar = 20 lm. Cells are representative within a population with independent experiments repeated four times. (B) Upper panel: Immunocytochemical detection of myc immunoreactivity allowed detection of the N12S GPR61 in unpermeabilized cells indicating protein expression in the cell membrane (red immunofluorescence). Subsequent permeabilization of cells followed by re-immunolabeling allowed visualization of myc-immunoreactive protein expressed throughout the cell (green immunofluorescence). DAPI stain (blue fluorescence) was used to visualize the cell nuclei. When the cell images were combined, immunoreactive protein expressed in the cell membrane appears yellow, whereas intracellular immunoreactive protein appears green. Treatment of the cells with tunicamycin (1.0 lgÁmL À1 , 48 h) resulted in the reduced level of cell membrane myc immunoreactivity shown as reduced levels of red staining. Lower panel: The same as in the upper panel but the intracellular staining following the permeabilization was performed using anti-GPR61 sera, and the resulting immunoreactivity appears green. The scale bar = 20 lm. Cells are representative within a population with independent experiments repeated four times. GPR61 identified bands of immunoreactivity consistent with the size of the predicted molecular weight of the myc-tagged GPR61 receptor~53 kDa (Fig. 2). The stably transfected cells also gave rise to a secondary band at about 110 kDa, which may suggest the formation of a dimer. Addition of tunicamycin (1.0 lgÁmL À1 ) to the cell culture medium for 48 h reduced consistently the apparent molecular weight of resulting myc-tagged GPR61 immunoreactivity by 1-2 kDa (Fig. 2), which was not apparent for the control protein GAPDH. This was further investigated by the mutation of the predicted N-glycosylation site in the N terminus of the myc-tagged GPR61 (N12), which also resulted in the arising protein having a reduced molecular weight of the predominant immunoreactive species by 1-2 kDa compared with the nonmutated protein. Tunicamycin-treated myctagged GPR61 and myc-tagged N12S cell lysates showed the same myc immunoreactivity pattern. These results indicate that the myc-tagged GPR61 is N-glycosylated.

Immunocytochemistry
Immunocytochemical studies on the transfected fixed HEK293 performed with either anti-myc or anti-GPR61 sera confirmed that myc-tagged GPR61 is expressed both at the surface and inside the cells (Fig. 3A,B). Cells treated with tunicamycin displayed considerably reduced levels of myc-tagged GPR61 immunoreactivity when the cells were stained with antimyc antibody before permeabilization with no apparent difference in the intracellular staining between treated and untreated cells. When the N-glycosylation site of myc-tagged GPR61 was disrupted (N12S), the staining corresponding to extracellular epitope in the mutant was similar to that of the nonmutated protein. However, following the tunicamycin treatment, the myctagged N12S also showed markedly reduced levels of surface myc staining, when compared with untreated cells. These results point toward the lack of a direct role for N-glycosylation of the myc-tagged GPR61 protein in the cell membrane trafficking of this protein. Under the same conditions, no immunofluorescence was detected when preimmune sera replaced the primary sera (data not shown). The distribution of intracellular staining revealed by either myc antibody or the anti-GPR61 antibody was near identical, indicating that these antibodies target the same protein.

Flow cytometry
Flow cytometric analysis of expression of myc-tagged GPR61 and N12S in the transfected HEK293 cells gave comparable results to immunocytochemistry (Fig. 4A) but allowed better quantification of the immunoreactivity.
As opposed to the immunocytochemical method, nonfixed cells were used in order to minimize the risk of cell permeabilization and prevent any intracellular staining. Using flow cytometry, we have demonstrated that both nonmutated and N12S forms of GPR61 were transported to the cell membrane and their cell membrane expression was reduced by approximately 40% following tunicamycin treatment (Fig. 4B).
Expression of GPR61 in human hippocampus GPR61 immunoreactivity was detected at different levels across hippocampal subfields (Fig. 5A-C). The GPR61 protein was relatively highly expressed in cells with the morphology of pyramidal neurons within subfields CA1, CA2, and CA3 of the hippocampus, and at lower levels in the granule cells of the dentate gyrus (DG) and large neurons in CA4 subfield with the morphology of GABAergic interneurons (Fig. 5A). Immunoreactivity was not apparent when preimmune sera exchanged the anti-GPR61 sera.
Expression of GPR61 in immune cells GPR61 mRNA expression was evident in human PBMCs with no real change in expression following activation of the cells with PHA (DC t = 28.52 and 29.93, respectively, Fig. 6). GPR61 expression was quantified by flow cytometry and was evident in all the investigated cell subsets at similar levels ( Fig. 7B-E).

Discussion
GPR61 is an orphan GPCR with little information concerning a role and very few published reports of protein expression patterns. GPR61 mRNA expression is relatively high in brain, leukocytes, and testis [2].
In this work, we have assessed the impact of N-glycosylation on the cellular expression of this GPCR in the stably transfected HEK293 cells. N-glycosylation has been shown to have a major role in cell trafficking and protein folding [16]. By the use of the N-glycosylation inhibitor, tunicamycin, and also the generation of a non-N-glycosylated mutant, N12S GPR61, it was evident that GPR61, when expressed in human cells, is prone to N-glycosylation. However, our results also indicate that while N-glycosylation of GPR61 is not required for insertion into the cell membrane, per se, nonselective inhibition of all N-glycosylation does prevent GPR61 insertion into the cell membrane, suggesting that N-glycosylated 'chaperone' proteins support GR61 membrane trafficking, which become nonfunctional when N-glycosylation is inhibited. Given the difficulty in identifying a functional activity for GPR61, it would be tempting to speculate that the receptor may function as a heterodimer and the delivery of the heteromeric dimer to the cell membrane was dependent on N-glycosylation of GPR61's partner GPCR. One of the potential candidates has been forwarder in the most recent paper in which it was suggested that GPR61 and also other members of its cluster, GPR62 and GPR135, may form a heterodimer with melatonin MT2 receptor upon overexpressing both receptors [9].
The fact that GPR61 is subject to N-glycosylation shows that it undergoes the same processes as many other GPCRs [14]. The impact of N-glycosylation on a membrane expression and a structure of ligand-binding domain has been shown for several GPCRs, with the examples including 5-HT 5A [17], b2-adrenergic [18], AT1 angiotensin [14], or B2-bradykinin [19].
There are a number of GPCR-interacting proteins that, for example, influence the surface trafficking and receptor signaling, and belong predominantly to heat shock protein (Hsp), RAMP, and PDZ-domain families. Some of these interacting proteins (e.g., RAMP2) are subject to N-glycosylation [20]. Presumably, other components of the machinery that are active in GPR61 cell membrane trafficking can also be impacted.
In order to be able to predict potential cellular functions of GPR61, we have investigated expression in human native tissues and cells with cellular resolution; previous reports of GPR61 expression merely reported expression by PCR, which showed relatively high levels of GPR61 mRNA in human brain, leukocytes, and testis [2]. Similarly, GPR61 mRNA expression was found to be at relatively high or moderate levels in mouse CNS (hypothalamus, olfactory bulb, striatum, and hippocampus) and testis [21]. In this study, we have used two antibodiesa goat polyclonal antibody that recognizes the C terminus (H-Cys-Ser-Asp-Ser-Tyr-Leu-Arg-Pro-Ala-Ala-Ser-Pro-Arg-Leu-Glu-Ser-OH) of GPR61 protein and a mouse monoclonal antibody recognizing myc-tag added to the N terminus of the GPR61 receptorto study the expression of native and myc-tagged GPR61 protein, respectively. In this study, we show that these two antibodies work effectively in immunocytochemistry and flow cytometry assays. Immunocytochemical staining of myc-tagged GPR61-transfected HEK293 cells demonstrated that these two antibodies indeed target the same protein. Additionally, the anti-myc antibody was used in western blot studies where the polyclonal goat antibody targeting the native protein failed to give satisfactory results. GPR61 protein expression was evident in the human hippocampus; hippocampal GPR61 immunoreactivity was widely expressed in the hippocampus at differing levels. Strong immunoreactivity signals were evident in the CA1, CA2, and CA3 subfields of the hippocampus associated with cells often displaying the morphology of pyramidal neurons. More moderate expression was detected in the DG and CA4 subfields. Hippocampal GPR61 expression in the hippocampus, particularly when associated with pyramidal neurons, suggests an involvement of this receptor in higher brain functions, such as learning, memory, and cognition [22,23].
Our study also revealed that human PBMCs express GPR61 protein (and also confirming the expression of mRNA from our studies and reports in the literature; [2]). We subsequently investigated subsets of human Specificity of GPR61 antisera was tested on HEK293 stably expressing myc-GPR61. Blueuntransfected HEK293 cells stained with preimmune sera; orangeuntransfected HEK293 stained with GPR61 antisera; green -HEK293 cells expressing myc-GPR61 stained with preimmune sera; red -HEK293 cells stably expressing myc-GPR61 stained with GPR61 antisera. (B) CD4+ T cells, (C) CD8+ T cells, (D) CD19+ B cells, (E) CD14+ monocytes. PBMCs were isolated from healthy donors and stained with cell surface markers specific for each subset. Cells were then permeabilized and the GPR61 immunoreactivity was assessed by staining with GPR61 antisera (blue) or preimmune control serum (red). The figure shows a representative example from three independent experiments.
PBMCs using flow cytometry and demonstrated expression in the CD4+, CD8+, CD14+, and CD19+ cell subsets isolated from blood from healthy volunteers, although these subsets appeared to express similar levels of the receptor. Examples of other relatively uniformly expressed membrane receptors in leukocytes include b-adrenergic and serotoninergic receptors [24]. GPCRs can play a major role in functioning and the development of immune responses, and many GPCRs have been reported to take part in transcriptional regulation [25].
Perhaps more interestingly, within the CD4+ subset, expression of GPR61 was higher in Th17 cells compared to Th1 cells and significantly higher than in resting CD4+ T cells. Th17 cells have been intensively studied in recent years since their discovery in early 2000s. These cells are a lineage of CD4+ T cell that produces IL-17 and appears to have a pathophysiological role in certain inflammatory diseases (e.g., multiple sclerosis, rheumatoid arthritis, psoriasis). It has been demonstrated that a shift from Th1 to Th17 phenotype may be modified by GPCRs [26]. On the other hand, antagonizing another GPCR -EP4 receptor for E2 prostaglandininhibited Th17 expansion and was reported as effective in contact hypersensitivity, EAE, and arthritis models [27,28]. Given the lack of reports about physiological effects mediated by GPR61, a potential role in Th17-dependent immunity and autoimmunity may warrant further investigation.
To conclude, we are reporting for the first time that GPR61 protein is subject to N-glycosylation, which is consistent with many other GPCRs. In addition, this membrane GPCR is expressed in the human brain (hippocampus) and in T cells, B cells, and monocytes with higher levels of protein expression in IL17-producing CD4+ T cells; such expression may help in the search for cellular functions mediated by this receptor, which may forward the receptor as a potential therapeutic target.
supported by the Medical Research Council (MRC Grant G0900580). The graphical abstract figure was partly produced using Prottervisualize proteoforms [29].
Author contributions GG, AJC, SJC, JWI, HP, and NMB supervised the study; PK, HA, SY, GG, and NMB designed experiments and analyzed data; PK, HA, and SY performed experiments; PK, HA, GG, SJC, and NMB wrote the manuscript; all authors approved the final version of the manuscript.