1 Department of Medicine, University of Cambridge, Cambridge, U.K.
2 Department of Clinical Biochemistry, University of Cambridge, Cambridge, U.K.
3 Department of Public Health and Primary Care, University of Cambridge, Cambridge, U.K.
4 CVGI Discovery, AstraZeneca Pharmaceuticals, Macclesfield, U.K.
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ABSTRACT |
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The neuropeptide prolactin-releasing peptide (PrRP) and its cognate G-protein-coupled receptor, GPR10, were initially identified as possible regulators of prolactin release from the anterior pituitary lactotroph. Subsequently, however, some doubt has been cast on the assertion that the main physiological role of PrRP and its receptor is in the control of prolactin release. Both neuroanatomical studies of the ligand and its receptor, as well as the physiological responses to central administration of PrRP, suggest roles in other processes, such as feeding behavior and the central control of blood pressure (1,2). The anorectic effect of PrRP has been demonstrated by the dose-dependent reduction in nocturnal food intake that follows a single intracerebroventricular (ICV) injection of PrRP into free-moving male rats. In 24-h-fasted rats, ICV PrRP can also inhibit food intake when compared with ICV saline (1). A role for PrRP in the central control of blood pressure is suggested by the finding of a highly significant elevation in mean arterial blood pressure observed in conscious, unrestrained male rats following a single ICV injection of PrRP in comparison with their saline-treated controls (2). To date, there are no reported human genetic studies of PrRP or GPR10 in relation to obesity or blood pressure. We therefore undertook mutation detection studies of these two genes in 94 subjects with severe early-onset obesity.
Eight polymorphic sites were found in GPR10 and four in PrRP. Two of the GPR10 polymorphisms (V283I and P305L) resulted in amino acid changes; all of the variants in the PrRP gene were silent (Table 1). V283I and P305L were found at similar allele frequencies (1 and 7%, respectively) in normal-weight Caucasians. Thus, major loss-of-function mutations in either PrRP or its receptor do not appear to be a common cause of severe human obesity.
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Neither polymorphism showed any association with BMI (Table 2), fasting glucose, insulin, triglycerides, or cholesterol (data not shown). However, significant associations between C914T and diastolic blood pressure (P < 0.01) and between G-62A and C914T and systolic blood pressure (P < 0.05) were found (Table 2). Blood pressure was higher in carriers of the -62A allele than in noncarriers. Similarly, those who were homozygous for the C914 allele had higher blood pressure readings than carriers of the 914T allele. These findings are consistent with the observed pattern of linkage disequilibrium between these two SNPs.
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The associations found between GPR10 polymorphisms and blood pressure are intriguing and deserve further study in independent populations. How might PrRP/GPR10 influence blood pressure? PrRP elevates blood pressure when administered ICV (2). PrRP is highly expressed in areas of the brain known to be important in the control of cardiovascular function, most notably the A1 and A2 areas of the caudal medulla, where PrRP immunoreactive neurones strongly costain with tyrosine hydroxylase (6). GPR10 is encoded on human chromosome 10q25.3q26.1 (7). While this is not a region that has been implicated in major genome-wide scans in human hypertension, it is notable that there is a major quantitative trait locus for blood pressure in rats on chromosome 1, in the region syntenic to human 10q2526.
We conclude that genetic variation in the G-protein-coupled receptor GPR10 may have an influence on human blood pressure. As is always the case with observations of this nature, replication studies in other large populations is a priority to determine the consistency of the genetic association.
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RESEARCH DESIGN AND METHODS |
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The MRC Ely Study is a prospective population-based cohort study of the etiology and pathogenesis of type 2 diabetes and related metabolic disorders (3,4). It is an ethnically homogeneous Caucasian population in which phenotypic data have been recorded on individuals both at the outset and after 4.5 years. All subjects were between 40 and 65 years of age at baseline. This cohort was recruited from a population sampling frame with a high response rate (74%), making it representative of the general population for this area of Eastern England. Of the 1,084 individuals studied, 29 (2.7%) had previously undiagnosed diabetes and 165 (15.2%) impaired glucose tolerance.
Genetics.
Genes were amplified from genomic DNA by PCR. Genomic DNA was isolated from whole blood using a QIAamp blood kit (Qiagen, London). PCR was performed using BioTaq (Bioline, London) and carried out as recommended by the manufacturer. Thirty-five cycles (30 s at 96°C, 40 s at 60°C, and 40 s at 72°C) were performed using a PTC-225 Peltier Thermal Cycler (MJ Research, Watertown, MA).
Following digestion, gel electrophoresis was performed using 3% (wt/vol) agarose gels (Gibco BRL, Paisley, U.K.) containing ethidium bromide and the pattern of bands were visualized and recorded after exposure of the gel to ultraviolet radiation. Sequencing was carried out using BigDye terminator chemistry (Perkin-Elmer, Beaconsfield, U.K.) and electrophoresed on an ABI 377 automated DNA sequencer (Perkin-Elmer, Foster City, CA). G-62A was genotyped by PCR amplification of the fragment containing this polymorphism, followed by digestion with the restriction enzyme BstN I (New England Biolabs, London), according to the manufacturers protocol. C914T was also typed following generation of a forced restriction enzyme site. Digestion of the PCR product was performed with the restriction enzyme SacI (New England Biolabs). The primers used in the PCR and sequencing and genotyping reactions are listed in the online appendix (http://diabetes.diabetesjournals.org).
Functional analysis of GPR10 variant.
An expression construct was formed by cloning the human GPR10 receptor cDNA into pcDNA 3.1 (Stratagene, La Jolla, CA). After verification by direct sequencing of the clone, mutagenesis of the construct to yield the 305L and 306STOP GPR10 receptor mutants was performed using the Quick Change site-directed mutagenesis kit (Stratagene) following the manufacturers protocol. HEK 293 cells were transfected with each of these three constructs using Lipofectamine (Gibco-BRL), as recommended by the manufacturer, and incubated in G418 (Gibco-BRL)-containing media for 4 weeks.
Clones (>100) derived from each transfection were pooled into populations and incubated in varying concentrations of PrRP and tested for differences in their intracellular signaling capacity through GPR10 using the FLIPR, as described (9). Each concentration of ligand was tested in quadruplicate. Briefly, cells were plated out in cell media (DMEM, 10% [vol/vol] FCS, 1% [vol/vol] penicillin/streptomycin, 1% [vol/vol] glutamine, and 1 mg/ml G418 [Gibco-BRL]) at 50,000 cells/well in Biocoat poly D-lysine 96-well black/clear plates (Fred Baker, Runcorn, U.K.) 24 h before use. Cells were incubated overnight at 37°C in a humidified tissue culture incubator set at 37°C in 5% CO2. One hour before beginning the assay, the cells were loaded with 100 µl assay buffer (HBSS, 0.02 mol/l HEPES, 1 µg/ml BSA, 2 mmol/l CaCl2, and 75 µg/ml probenecid, pH 7.4) (Sigma, St. Louis, MO) containing 0.2% (vol/vol) Fluo-4 AM and 0.2% (vol/vol) pluronic acid (Molecular Probes, Eugene, OR) and then placed back in the tissue culture incubator. Cells were then washed three times with 200 µl of assay buffer, leaving 100 µl residual volume after the final wash. PrRP-31 (Phoenix Pharmaceuticals) was made up at three times the required final test concentration in 100 µl assay buffer in a 96-well plate. Test plate fluorescence was then measured by the FLIPR every second for 10 s before adding PrRP-31. Fluorescence was measured every second for a further 80 s. PrRP-31 was added in a volume of 50 µl. The maximum change in fluorescence in each well measured between 10 and 80 s was corrected for the baseline fluorescence measured over the first 10 s before addition of test PrRP-31. This baseline fluorescence is dependent on cell number and dye loading efficiency and is therefore a reasonable means by which to normalize the data.
Statistical methods.
Linkage disequilibrium test and haplotype analyses were performed using the expectation-maximization algorithm. Association analyses between the genotype and the phenotype were performed using the MIXED procedure in the Statistical Analysis System (SAS for Windows, version 8.2); this allows incorporation of unbalanced repeated data, which improves the power of the study. Means were adjusted for age and sex when BMI was the outcome and for age, sex, and BMI when blood pressure was the outcome. Statistical significance was determined in the G-62A genotype by comparing the means for each of the three genotype groups. For the C914T genotype, only two genotype groups existed; therefore, the P value reflects the difference between these two groups.
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ACKNOWLEDGMENTS |
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FOOTNOTES |
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Received for publication 9 December 2002 and accepted in revised form 10 February 2003.
Additional information for this article can be found in an online appendix at http://diabetes.diabetesjournals.org.
FLIPR, fluorometric imaging plate reader; ICV, intracerebroventricular; PrRP, prolactin-releasing peptide.
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REFERENCES |
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