The mu-opioid receptor (OPRM1) A118G polymorphism underpins different pain sensitivity and opioid-analgesic outcome with unclear effect on the descending pain modulatory system (DPMS). Primary dysmenorrhea (PDM), the most prevalent gynecological problem with clear painful and pain free conditions, serves as a good clinical model of spontaneous pain. The objective of this imaging genetics study was therefore to explore if differences in functional connectivity (FC) of the DPMS between the OPRM1 A118G polymorphisms could provide a possible explanation for the differences in pain experience. Sixty-one subjects with PDM and 65 controls participated in the current study of resting-state functional magnetic resonance imaging (fMRI) during the menstruation and peri-ovulatory phases; blood samples were taken for genotyping. We studied 3 aspects of pain experience, namely, mnemonic pain (recalled overall menstrual pain), present pain (spontaneous menstrual pain), and experimental pain (thermal pain) intensities. We report that G allele carriers, in comparison to AA homozygotes, exhibited functional hypo-connectivity between the anterior cingulate cortex (ACC) and periaqueductal gray (PAG). Furthermore, G allele carriers lost the correlation with spontaneous pain experience and exhibited dysfunctional DPMS by means of PAG-seeded FC dynamics. This OPRM1 A118G-DPMS interaction is one plausible neurological mechanism underlying the individual differences in pain experience.
The experience of pain and the clinical response to opioid analgesics varies among people. The analgesic effects of opioids are substantially mediated by the mu-opioid receptor (OPRM1) in the central nervous system1. A single nucleotide polymorphism producing an adenine (A)-to-guanine (G) substitution at codon118 (A118G) in the human OPRM1 gene is associated with reduced expression of the OPRM1 gene2, hypersensitivity to pain3, and an increased consumption of analgesics for clinical pain4.
The periaqueductal gray (PAG), enriched with opioidergic neurons1, acts as a critical hub in the neuraxis of the descending pain modulatory system (DPMS)5 that is pivotal for pain relief6. Nevertheless, to the best of our knowledge, no study has addressed how the OPRM1 A118G polymorphism modulates the DPMS to relate the individual pain experience. In the current imaging genetics study (using neuroimaging as an endophenotypic assay to evaluate genetic associations, with pain as an environmental stress) we investigated the neural network mechanisms of the OPRM1 A118G polymorphism for the central modulation of pain in otherwise healthy women with primary dysmenorrhea (PDM).
PDM, defined as menstrual pain without discernable organic causes, is the most prevalent gynecological problem with clear painful (menstrual phase) and pain free (e.g., peri-ovulatory phase) conditions and serves as a good clinical model of spontaneous pain7. PDM is considered as a genuine chronic pain condition8 because the neural substrates of pain matrix may be altered in long-term PDM in the context of glucose metabolism, regional homogeneity and activity, state- and trait-related structural changes9,10,11,12,13. State-related changes are menstrual pain-primed, whereas trait-related changes exist even without symptoms. Alterations of regional gray matter volume in PDM substantially involved the DPMS (PAG, insula, ACC/medial prefrontal cortex [mPFC], and etc.)10. It is suggested that the maladaptive functional connectivity (FC) in the DPMS (PAG-ACC/mPFC and PAG-supplementary motor area [SMA]) in young PDM subjects may underpin the central susceptibility to subsequent development of various chronic pain disorders later in life7. Such PAG-ACC/mPFC hypo-FC is a co-terminal to many functional pain disorders, while altered SMA FC is common in chronic pelvic pain disorders7,14. Notably, there may even be developmental attributions for PDM owing to its association with a high prevalence of normal variants15.
Using PAG seed-based FC approach, studies have revealed abnormal DPMS neurodynamics in patients with chronic low back pain16, chronic myofascial pain17, fibromyalgia18, migraine19, and PDM7; the alterations of PAG-seeded FC dynamics relate patients’ pain experience. We further reported that the PAG-seeded DPMS FC patterns in pain-free controls are altered in women with PDM in a genotype-specific manner20. We set out in the current study to investigate the effect of OPRM1 A118G polymorphism on the PAG-seeded DPMS FC dynamics throughout the menstrual cycle and correlate different aspects of pain experience with the PAG-seeded FCs in the PDM subjects. Here, we studied 3 aspects of pain experience, namely, mnemonic pain (recalled overall menstrual pain), present pain (spontaneous menstrual pain), and experimental pain (thermal pain) intensities. We hypothesized that the OPRM1 A118G polymorphism may be associated with disparate PAG-seeded FCs (networks) in the DPMS that may explicate the individual differences in pain experience.
Demographic data and baseline information
Sixty-one PDM subjects (AA n = 26, AG n = 31, GG n = 4; 23.2 ± 2.27 years of age) and 65 age- and education-matched healthy female controls (AA n = 23, AG n = 36, GG n = 6; 23.8 ± 2.36 years of age) of the same Chinese ethnicity were eligible for imaging genetics studies. No significant differences between the PDM subjects and the controls were detected for the OPRM1 A118G polymorphism (p = 0.660) and the A118G-genotype distribution did not deviate from the Hardy–Weinberg equilibrium in both PDM (p = 0.19) and control group (p = 0.13). AG heterozygotes and GG homozygotes were considered as a single genotype (“G allele carriers”) based on their similar clinical characteristics4. There were no significant group or genotype differences with regard to age, years of menstruation, average days of 1 menstrual cycle, or Edinburgh Handedness Inventory scores (Table 1).
All 61 PDM subjects in this neuroimaging study had a long history of menstrual pain (mean ± SD = 8.95 ± 2.82 years), with the pain lasting approximately 1 to 3 days during one menstrual cycle (mean ± SD = 1.93 ± 0.79 days). Thirty-four PDM subjects (55.7%) reported absences from school or work as a result of debilitating menstrual pain, and 28 PDM subjects (45.9%) used over-the-counter analgesics on occasion. There was no significant genotype difference with regard to history of menstrual pain (p = 0.819), duration of menstrual pain (p = 0.931), absences from school or work (p = 0.432), or analgesics taken (p = 0.813).
The mnemonic experience (mean ± SD = 34.84 ± 13.92) and the present experience (mean ± SD = 31.66 ± 13.02) of menstrual pain, as assessed by scores on the McGill Pain Questionnaire, confirmed that the PDM subjects experienced moderate to severe menstrual pain. The pain rating index (PRI) of present pain was significantly lower than that of mnemonic pain (p = 0.039; mnemonic pain is usually rated higher than present pain7,21). Notably, G allele carriers rated present pain sub-significantly higher than AA homozygotes under similar mnemonic pain experience (Table 1).
Serum gonadal hormone measurements
There were phase differences for all 3 gonadal hormones. No group or OPRM1 genotype difference was noted (Table 2). As gonadal hormones may affect the resting-state FC22,23,24, the hormone fluctuations were regressed out as covariates of non-interest during the subsequent image processing.
Thermal quantitative sensory test
The PDM subjects had lower heat-pain thresholds in the C7 (remote control area; significant) and T11 dermatomes (referral area of menstrual pain; sub-significant), suggesting central sensitization throughout the menstrual cycle as previously reported in white populations25,26,27. No significant genotype or menstrual cycle difference was noted (Table 3).
PAG-seeded FC maps for the between-genotype and between-group differences
In the overall between-genotype FC comparisons, G allele carriers showed decreased PAG-ACC/mPFC and PAG-dorsolateral prefrontal cortex (dlPFC) FCs compared with AA homozygotes. Among the control group, G allele carriers showed decreased PAG-ACC, PAG-dlPFC and PAG-temporal lobe FCs compared with AA homozygotes. Among the PDM subjects, G allele carriers showed decreased PAG-ACC/mPFC, -orbitofrontal cortex and -superior parietal lobule FCs compared with AA homozygotes at a lower threshold (uncorrected p = 0.005, voxels >60). Only among the G allele carriers, PDM subjects showed increased PAG-SMA FC compared with the controls (Fig. 1, Table 4).
Correlation analysis between functional connectivity and the pain rating index of the McGill Pain Questionnaire
During the menstruation, the AA homozygous PDM subjects exhibited positive correlations between their present experience of menstrual pain and PAG-seeded FC in the ACC, insula, secondary somatosensory cortex (S2), subthalamic nucleus, and cerebellum (Table 5). However, the PDM subjects with G allele showed no correlation between PAG-seeded FC and their experience of menstrual pain, either present or mnemonic.
Correlation analysis between functional connectivity and the heat-pain threshold of the quantitative sensory test
During both phases, only the PDM subjects with G allele exhibited negative correlations between PAG-cuneus FC and their heat-pain thresholds over both C7-dermatome and T11-dermatome (Table 6).
Individual differences in pain experience may stem from genotype-laden different pain processing and neuromodulatory mechanisms in the brain, especially the DPMS. Here we report that AA homozygotes, in comparison to G allele carriers, exhibited increased PAG-ACC FC that correlated with their spontaneous menstrual pain experience. The AA homozygous PDM demonstrated an active cortical modulation, whilst the PDM subjects with G allele showed dys-regulated DPMS. This OPRM1 A118G-DPMS interaction can be one plausible neurological mechanism underlying the individual differences in pain experience.
In the overall between-genotype FC comparisons, G allele carriers (vs. AA homozygotes) showed hypo-FCs between the ACC, mPFC and dlPFC with PAG during menstruation (Fig. 1a). All of these FCs participate in the cortical modulation of pain6,28. The findings indicate an innately decreased endogenous modulation in G allele carriers even among the healthy subjects (Fig. 1b). This view is corroborated by the reported observation that G allele carriers require more self-administered analgesics after surgery4,29.
Using a relatively liberal statistics (uncorrected p = 0.005, voxels >60; compromising with relatively small sample size of AA homozygous PDMs n = 26 vs. G allele carrier PDMs n = 35) to unravel subtle genetic effect yet important information from the subset analyses, we observed significant differences in the between-genotype comparison among PDM subjects (Fig. 1c). The PAG-ACC, -mPFC, -orbitofrontal cortex, and -superior parietal lobule FCs are all known to substantially participate in the cortical modulation of pain28. The findings from the subset analyses of PDM subjects were corroborative to those from between-genotype comparisons of the controls (Fig. 1b) and overall subjects (Fig. 1a); all these between-genotype comparisons (overall, controls, and PDMs, respectively) showed consistent PAG-ACC hypo-FC in G allele carriers (Table 4). The ACC, enriched with opioidergic neurons30, is pivotal for the DPMS with respect to placebo, opioid analgesia31,32, and distraction from pain33,34. Therefore, the PAG-ACC FC is likely to be one plausible neurological mechanism underlying the OPRM1 A118G polymorphism-associated genetic differences in pain experience. Our reasoning is supported by the correlations between present pain experience and the PAG-ACC FC only in the AA homozygous PDM subjects during menstruation, but not in the PDM subjects with G allele (Table 5). Collectively, our data suggest an active cortical modulation for present menstrual pain and may explain why AA homozygotes rated their present pain experience sub-significantly lower than G allele carriers.
In the between-group comparisons for each genotype, only the G allele carriers with PDM exhibited increased PAG-SMA FC during menstruation (Fig. 1d). Increased SMA activation has been noted in G allele carriers compared with AA homozygotes during painful electrical stimulation35. Such PAG-SMA FC is a co-terminal to many chronic pelvic pain disorders and may implicate a dysfunctional DPMS involving the medial motor cortex and PAG7,14. The findings suggest that G allele carries can be associated with higher vulnerability for the development of chronic pain. Furthermore, the negative correlations between the PAG-cuneus FC and experimental heat-pain thresholds over both C7- and T11-dermatomes throughout their menstrual cycle (trait correlation; Table 6) imply that the PAG-cuneus FC could predict the pain sensitivity. It has been suggested that the cuneus may have a connection to the PAG because stimulation of the area in rats leads to descending pain alleviation36, and the PAG-cuneus FC is engaged for pain modulation in PDM subjects7. However, the negative correlations in G allele carriers implicate maladaptive neuroplasticity. It is noteworthy that G allele carriers exhibited no correlation between their PRI and PAG-seeded FC. Collectively, the absence of state correlations and the presence of stationary trait correlations in G allele carriers may implicate subclinical dys-regulated pain modulation.
Unlike some previous genetic studies on the OPRM1 A118G polymorphism, we did not observe differences in the heat-pain threshold. There are several explanations for these inconsistencies in the existing literature, including differences in sex proportion (sex by genotype interaction emerges for heat pain37), pain modalities (neither electrical3 nor pressure37 pain stimulation), and ethnicity (Asians are different from Caucasians in the G allele variability38 and in the phenotype of the OPRM1 A118G polymorphism39). As the penetrance of genes can be greater at the level of brain biology than at the level of behavior40, neuroimaging bridges the mechanistic gap between gene and behavior41. Neuroimaging may be more sensitive than behavioral measurements, i.e., the neuroimaging findings can be sub-clinical without conspicuous behavioral manifestation42; therefore, the PDM subjects with G allele may show altered FC, but without conspicuous behavioral differences in their heat-pain thresholds.
Our study depicts that the OPRM1 A118G polymorphism influences the DPMS FC dynamics during painful menstruation phase (state-related change) in the PDM subjects, but not during the pain-free peri-ovulatory phase (trait-related change), positing menstrual pain as a potential attributor of epigenetic regulation (Fig. 1 and Table 4). It has been reported that epigenetic modifications (DNA methylation in the frontal cortex) mostly happen during the period of adolescent and become stable in adults43. It is tempting to speculate that early PDM experiences might invoke epigenetic regulation of OPRM1 A118G polymorphism, affect the frontal DPMS with long-term sensitization, and incur maladaptive neuroplasticity that eventually might lead to various functional pain disorders later in life in the vulnerable female subjects7. It should be born in mind that vulnerability to an illness, e.g., PDM, may stem not only from a single single-nucleotide polymorphism effect but also the interactions and contributions of multiple genes44. In line with this, we have recently reported that the BDNF Val66Met polymorphism modulates the FC dynamics in the DPMS and might substantiate individual vulnerability to the development of chronic functional pain in women with PDM20. Whether there is a gene–gene interaction between the OPRM1 A118G polymorphism and the BDNF Val66Met polymorphism can be of high interest in further studies.
Multi-factorial models (including gene, sex, age, ethnicity, life event, psychology, and etc.) may underlie individual differences that make effective standardized-treatment difficult; however, studies have reported personalized opioid use by prediction formulas containing several genetic polymorphisms within or close to the OPRM1 gene45. Our data also pinpoint the importance of individualizing analgesic therapy to optimize medical treatment for pain relief46. Given that the PAG is substantially involved in both placebo effects and motor cortex stimulation for pain alleviation6,47, AA homozygotes with higher functional expression of the DPMS may have better endogenous and exogenous modulations of pain. Our data suggest that conventional analgesic treatment or noninvasive brain stimulation might be good choices for chronic pain patients who are AA homozygotes. In contrast, analgesics combined with more aggressive “multimodal” pain alleviation techniques might be ideal choices for the chronic pain patients who are G allele carriers46.
To our knowledge, this is the first study that provides novel insight into the hitherto unexplored neurodynamic influences of the OPRM1 A118G polymorphism on the FCs of PAG-based DPMS. Such genetic variations shape the functional organization of DPMS and may predict or underpin the differential efficacy of analgesics (responder or non-responder)48, and eventually may also attribute to the vulnerability to the development of chronic pain late in life of PDM subjects20. Our preliminary report invites future studies of larger sample size for the verification and to further explore whether such OPRM1 A118G polymorphism-FCs of PAG-seeded DPMS interactions for individual pain experience can be generalized to other chronic functional pain disorders.
Materials and Methods
All participants were recruited from Internet advertisements from August 2011 to August 2015. Originally, 153 PDM subjects and 151 controls were screened using telephone and in-person structured interviews regardless of case or control status. Two PDM subjects and 7 controls were then excluded after rigorous screening according to the exclusion criteria and one of the following factors: inconsistent pain intensity, left-handedness, premenstrual dysphoric disorder, or head injury. After entering the integrated behavioral and multimodal imaging genetics studies (magnetic resonance imaging and magnetoencephalography), 8 PDM subjects were excluded owing to pelvic abnormalities on ultrasonography scans; 2 PDM subjects and 2 controls were excluded owing to an irregular menstrual cycle; 1 PDM subject and 1 control were excluded owing to a prolonged menstrual cycle; 17 PDM subjects and 2 controls were excluded owing to incidental brain findings15; 57 PDM subjects and 53 controls were excluded because they were unwilling to complete the entire series of genetic, hormonal, behavioral, and multimodal neuroimaging studies, which would resulted in incomplete datasets; 2 PDM subjects and 12 controls were excluded because of abnormal hormone levels (possibly due to sampling and technical errors); and 3 PDM subjects and 9 controls were excluded owing to head motion (>2 mm) or rotation (>2°) during the scan. Eventually, 61 PDM subjects and 65 controls were eligible for neuroimaging analyses in this study (entire protocol completed).
The inclusion criteria for the PDM subjects were the following: 1) a regular menstrual cycle of approximately 27–32 days; 2) a history of menstrual pain longer than 6 months; 3) an averaged menstrual pain under regular treatment with a rating that was higher than 4 on a verbal numerical scale (VNS, 0 = not at all, 10 = the worst imaginable pain) over the last 6 months; and 4) right-handedness, as confirmed by the Edinburgh Handedness Inventory. The inclusion criteria for the healthy female controls were similar to those for the PDM subjects, except that the controls had no pain whatsoever during menses (VNS = 0). The exclusion criteria for all the participants were as follows: 1) using oral contraceptives, hormonal supplements, Chinese medicine, or any centrally acting medication (e.g., opioid, anti-epileptics) within 6 months prior to the study; 2) pathological pituitary gland disease; 3) organic pelvic disease; 4) any psychiatric or neurological disorders; 5) any head injury with loss of consciousness; 6) immediate plans for pregnancy or a positive pregnancy test; 7) a history of childbirth; and 8) having a metal implant, a pacemaker implant, claustrophobia, or any contraindications in relation to magnetic resonance imaging (MRI). No analgesics had been taken by the subjects within 24 hours before the study. All PDM subjects were double-screened and diagnosed at a gynecology clinic by a gynecologist (H.T.C.) and received pelvic ultrasonography to exclude secondary dysmenorrhea caused by an organic pelvic disease such as endometriosis or adenomyosis. The study was conducted in accordance with the Declaration of Helsinki and was approved by the Institutional Review Board of Taipei Veterans General Hospital. All participants provided their written informed consent.
Blood samples for genotyping were collected during the initial examination, but genotypes of all participants were not known before the scanning session. MRI scans (T1 and resting-state fMRI images) were individually scheduled according to each subject’s first day of menstruation at two time points during the menstrual cycle: menstruation (days 1–3 of the menstrual cycle) and peri-ovulatory phase (days 12–16 of the menstrual cycle). Blood samples were collected at the same day and subjected to a gonadal hormone assay. For the detailed information of the genotyping and serum gonadal hormone measurements, please refer to our published paper7,20.
PDM subjects completed the McGill Pain Questionnaire during the initial examination (for mnemonic pain) and menstruation (for present pain); all participants completed the thermal quantitative sensory tests (for experimental pain) during menstruation and peri-ovulatory phase. For mnemonic and present pain, the PRI value in the McGill Pain Questionnaire was used to access menstrual pain experience since the scoring encompasses different dimensions of pain experience (i.e., sensory, affective, evaluative, and miscellaneous dimensions). For experimental pain, heat-pain threshold (as an index of pain sensitivity) was assessed by means of thermal quantitative sensory test.
Thermal quantitative sensory test
We performed thermal quantitative sensory testing according to the established protocol of an ascending limit approach for heat-pain thresholds49. Hot stimuli (TSA 2001-II, MEDOC, Israel) were administered to the bilateral peri-umbilical areas (T11-dermatome, referral area of menstrual pain) and forearm extensor areas (C7-dermatome, remote control area). The baseline temperature was set at 32 °C, and all the thresholds were obtained by a ramped stimulation method (1 °C/sec). The mean thresholds were calculated by averaging 3 consecutive measurements. The upper limit of the temperature was set at 50 °C.
Resting-state fMRI images were acquired using a 3.0 Tesla MRI scanner (Magnetom Trio Tim, Siemens, Erlangen, Germany) with a 12-channel head coil at National Yang-Ming University. High-resolution T1-weighted 3-dimensional structural images using a magnetization-prepared rapid-acquired gradient echo sequence (MPRAGE; TR/TE = 2530 ms/3.03 ms, flip angle = 70°, field-of-view = 224 × 256 × 192 mm3, matrix size = 224 × 256 × 192, in-plane resolution = 1 mm) and T2*-weighted gradient echo sequence (TR/TE = 2500 ms/30 ms, flip angle = 90°, field-of-view = 220 × 220 × 136 mm3, matrix size = 64 × 64 × 40, in-plane resolution = 3.4 mm [round-out], and 200 volumes per run) were performed to obtain high-resolution anatomical T1 images and fMRI images7. The participants remained awake during the scan (eyes open, head still but relaxed, without thinking about anything in particular). Head cushions and earplugs were provided to reduce head motion and noise, respectively.
Preprocessing was performed using the DPARSF toolbox (State Key Laboratory of Cognitive Neuroscience and Learning, Beijing Normal University, China) with Statistical Parametrical Mapping 8 (SPM8, Wellcome Trust Centre for Neuroimaging, London, http://www.fil.ion.ucl.ac.uk/spm) in Matlab. All functional images were subjected to slice timing, realignment for head-motion correction, co-registration against each individual’s anatomical image as well as normalization (nonlinear transformation) against the Montreal Neurological Institute (MNI-152) template. Subjects exhibiting any head motion of more than 2 mm or 2° were excluded from further processing50. The images were re-sampled to an isotropic 2 × 2 × 2 mm3 voxel size during the normalization step and then spatially smoothed using a 3D Gaussian kernel of 8 mm full-width at half-maximum. Linear trends were then removed from the resulting time series, and the time series was temporally band-pass filtered (0.01–0.08 Hz) to extract the low-frequency oscillations associated with spontaneous neuronal activity51.
Removal of physiological and scanner-related noise
The averaged time courses of the following nuisance variables or confounding artifacts were regressed out: 1) the six head-movement parameters computed based on rigid body translation and rotation during the realignment in SPM8; 2) the global mean signal (global signal regression); 3) the mean signal within the lateral ventricles; and 4) the mean signal within a deep white matter region (centrum ovale). The cerebrospinal fluid and the white-matter signals are thought to reflect fluctuations in non-specific regional correlations. We performed global signal regression because it can maximize the spatial specificity of positive resting-state correlations52, improve correspondence to anatomy53 and to electrophysiology54. The neuroscientific interpretation of anti-correlation has been challenged55, and global signal regression may cause a negative shift in the distribution of correlations53; therefore, we implemented a mask and addressed positive connectivity only in order to remove distortion after global signal regression56 as reported in our previously published work7,20.
Definition of PAG seed and PAG-seeded FC maps
The PAG seed (3-mm radius), centered at MNI coordinate [−4, −26, −14], was identified based on the published literature57,58. This seed is located within the ventrolateral PAG57 that is important for the opioid-mediated analgesia59. In healthy subjects, this region was activated during increased levels of heat-pain stimulation60, and was functionally connected to the key regions of the DPMS57. The mean time-series activity in the seed region of each subject was extracted. PAG-seeded FC maps were then generated. Each individual-level FC map obtained was then converted into a z-map using Fisher’s r-to-z transformation for second-level group analyses50.
Demographic information and psychophysiological measurements
SPSS Statistics 20.0 (SPSS Inc., Chicago, IL) was used for all of these analyses. The results were considered significant at p = 0.05 (two-tailed). The Hardy-Weinberg equilibrium of the OPRM1 genotype distribution in each group and the A118G-genotype distribution between two groups were assessed using the chi-square test. Normality was tested for all assessments, and only the PRI values in the McGill Pain Questionnaire were normality (p > 0.05). Therefore, a repeated-measures analysis of variance (ANOVA) of the McGill Pain Questionnaire scores was conducted to assess the main effects of OPRM1 genotype (AA homozygotes vs. G allele carriers) and pain-type (present vs. mnemonic), as well as the interaction between them. To assess the effects of groups (PDM vs. control) and/or OPRM1 genotype (AA homozygotes vs. G allele carriers), a Mann–Whitney U test was conducted for demographic characteristics, Edinburgh Handedness Inventory scores, durations of menstrual pain, serum hormone levels, and heat-pain thresholds. To assess the effect of menstrual cycle phase (menstruation vs. peri-ovulatory phase), a Wilcoxon signed-rank test was applied to serum hormone levels and heat-pain thresholds. Generally, the data met the assumptions of the statistical tests used, and the variance was similar between groups and OPRM1 genotypes.
A mixed-effects model of factorial design (2 factors: genotype and group) was employed to analyze the FC maps using SPM 8 (Wellcome Trust Centre for Neuroimaging, London, http://www.fil.ion.ucl.ac.uk/spm) for each phase. Gonadal hormones were regressed out as covariates of non-interest. Statistical maps (Fig. 1) were computed to identify changes in PAG-seeded FC for the following comparisons: 1) overall between-genotype comparison, 2) between-genotype comparisons for each group and 3) between-group comparisons for each genotype. PAG-seeded FC changes during menstruation (painful stage) in the comparisons were regarded as state changes, whereas changes during the peri-ovulatory phase (pain-free stage) or throughout the menstrual cycle were regarded as trait changes. Significance was thresholded at the uncorrected voxel level p = 0.005, followed by the FWE-corrected cluster level p = 0.05.
In the PDM group, the state correlation between the PRI of present pain and the PAG-seeded FC maps during menstruation was performed using a one-tailed two-sample t-test by the SPM. In contrast, the trait correlation between the PRI of mnemonic pain was similarly correlated with the PAG-seeded FC maps during the peri-ovulatory phase. We first entered the demeaned (in SPM) PRI values from present or mnemonic McGill Pain Questionnaire as regressors to identify brain regions with either positive or negative correlations with PAG-seeded FC in menstruation or peri-ovulatory phase7. Between-genotype comparisons were performed to identify regions where the correlation between PAG-seeded FC and the PRI was greater. Gonadal hormones were regressed out as covariates of non-interest. Significance was thresholded at the uncorrected voxel level p = 0.005, followed by the FWE-corrected cluster level p = 0.05.
For each phase, a one-tailed two-sample t-test was conducted to examine the correlation between the heat-pain thresholds and the PAG-seeded FC in the PDM group. Gonadal hormones were regressed out as covariates of non-interest. We first entered the demeaned (in SPM) heat-pain thresholds from the quantitative sensory test as regressors to identify brain regions with either positive or negative correlations with PAG-seeded FC in both genotypes. Between-genotype comparisons were performed to identify regions where the correlation between PAG-seeded FC and the heat-pain threshold was greater. Correlations during menstruation were regarded as state relationships, whereas correlations during the peri-ovulatory phase or throughout the menstrual cycle were regarded as trait relationships. Significance was thresholded at the uncorrected voxel level p = 0.005, followed by the FWE-corrected cluster level p = 0.05.
Because the SPM reports peak coordinates as identified within a confluent cluster, there can be multiple peaks that sit on different brain regions/areas (e.g., Brodmann area). We reported one representative peak for each region/area (e.g., in Table 4, dorsolateral prefrontal cortex and medial prefrontal cortex belong to a same cluster). Anatomical locations were determined according to probabilistic atlases of Harvard-Oxford Cortical Structural Atlas and Talairach Daemon Labels. To display 3D imaging, we used MRIcroGL for 3D rendering (Department of Psychology, University of South Carolina http://www.mccauslandcenter.sc.edu/mricrogl by Chris Rorden).
How to cite this article: Wei, S.-Y. et al. The OPRM1 A118G polymorphism modulates the descending pain modulatory system for individual pain experience in young women with primary dysmenorrhea. Sci. Rep. 7, 39906; doi: 10.1038/srep39906 (2017).
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This work was supported by Taipei Veterans General Hospital (V100D-001, V100D-001-1, V100D-001-2, V101C-152), Ministry of Science and Technology (NSC 100-2314-B-010-006-MY3, NSC 100-2629-B-010-001, NSC 101-2629-B-010-001, NSC 102-2629-B-010-001, MOST 103-2321-B-010-020), TVGH-NTUH joint research program (VN103-05, VN104-03, VN105-03), and The Aim for the Top University Plan of the Ministry of Education for National Yang-Ming University. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript. The authors thank all the participants in this study and extend particular appreciation to Chia-Yen Wu, Tzu-Ling Tseng, Yueh-Hua Chen, Ya-Yun Chen, and Pei-Shan Hsu for their technical and experimental help.
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