Abstract
Background
Non-cellular blood circulating microRNAs (plasma miRNAs) represent a promising source for the development of prognostic and diagnostic tools owing to their minimally invasive sampling, high stability, and simple quantification by standard techniques such as RT-qPCR. So far, the majority of association studies involving plasma miRNAs were disease-specific case-control analyses. In contrast, in the present study, plasma miRNAs were analysed in a sample of 372 individuals from a population-based cohort study, the Study of Health in Pomerania (SHIP).
Methods
Quantification of miRNA levels was performed by RT-qPCR using the Exiqon Serum/Plasma Focus microRNA PCR Panel V3.M covering 179 different miRNAs. Of these, 155 were included in our analyses after quality-control. Associations between plasma miRNAs and the phenotypes age, body mass index (BMI), and sex were assessed via a two-step linear regression approach per miRNA. The first step regressed out the technical parameters and the second step determined the remaining associations between the respective plasma miRNA and the phenotypes of interest.
Results
After regressing out technical parameters and adjusting for the respective other two phenotypes, 7, 15, and 35 plasma miRNAs were significantly (q < 0.05) associated with age, BMI, and sex, respectively. Additional adjustment for the blood cell parameters identified 12 and 19 miRNAs to be significantly associated with age and BMI, respectively. Most of the BMI-associated miRNAs likely originate from liver. Sex-associated differences in miRNA levels were largely determined by differences in blood cell parameters. Thus, only 7 as compared to originally 35 sex-associated miRNAs displayed sex-specific differences after adjustment for blood cell parameters.
Conclusions
These findings emphasize that circulating miRNAs are strongly impacted by age, BMI, and sex. Hence, these parameters should be considered as covariates in association studies based on plasma miRNA levels. The established experimental and computational workflow can now be used in future screening studies to determine associations of plasma miRNAs with defined disease phenotypes.
Electronic supplementary material
The online version of this article (doi:10.1186/s12920-015-0136-7) contains supplementary material, which is available to authorized users.
Keywords: BMI, Age, Sex, Circulating microRNA, miRNA, Association studies, Plasma, Blood
Background
MicroRNAs (miRNAs) are small ~22 nt long non-coding RNAs which play important regulatory roles by targeting mRNAs for degradation or mediating translational repression. Thus, they affect a wide range of physiological and pathophysiological processes including cell differentiation, proliferation, apoptosis, angiogenesis or inflammation [1, 2]. Besides their common intracellular localization, miRNAs are present in different body fluids, particularly in blood. The factors that determine the levels of extracellular miRNAs, e.g. in plasma, such as active secretion or passive release due to cell lysis as well as the functional roles of these plasma miRNAs are still under investigation. Non-cellular blood circulating microRNAs (in the remainder of this paper referred to as plasma miRNAs) are highly ribonuclease-resistant because they are either enclosed in membranous vesicles as apoptotic bodies and exosomes or localized in complexes with RNA-binding proteins (Ago2), high-density lipoproteins or nucleophosmin [3–5]. Recent studies have proposed a hormone-like role for circulating miRNAs in intercellular communication [3, 4]. The putative value of plasma miRNAs as predictive and diagnostic biomarkers motivated the recent large-scale profiling of these molecules in the context of many diseases, such as cancer, diabetes, multiple sclerosis, coronary artery disease or myocardial infarction [6–8]. A selection of 19 potentially informative plasma miRNAs was investigated by Zampetaki et al. [8] in a prospective, population-based study on cardiovascular disease. The study revealed associations between several miRNAs and the incidence of myocardial infarction and highlighted platelets as a major source for the plasma miRNA pool [8]. Few other population based studies were published on circulating miRNAs derived from blood cells [9] or serum [10]. Usually, the screening for candidate miRNAs has so far been performed on pooled or individual samples of cases and controls. Selected miRNAs have been measured by RT-qPCR in the entire sample or a sub-sample of the study cohort. Selection bias and co-morbidities might have affected the phenotype under investigation [11]. For instance, studies on miRNA levels detected in human plasma samples provided evidence for age-associated miRNA levels in blood [12, 13]. Such associations are almost certainly relevant in studies on age-related diseases such as cancer or cardiovascular disorders. Recently, the impact of age and sex on circulating miRNA was explored in peripheral blood using microarray technology [14]. This study highlighted the importance of age matching case-control studies whereas sex seemed to have a less pronounced effect on the miRNA levels [14]. The use of matched case-control cohorts or adjustment for age and sex is therefore warranted [11].
In the present study, we investigated plasma miRNAs prepared from human plasma using a reverse transcription-quantitative PCR (RT-qPCR) approach based on the Serum/Plasma Focus microRNA PCR Panel V3.M (Exiqon) which provides a higher sensitivity and specificity compared to array-based techniques [15]. We assessed the association of age, body mass index (BMI), and sex with miRNA levels in a sample of 372 individuals from the population based Study of Health in Pomerania (SHIP-TREND) applying stringent data pre-processing and taking into account technical as well as blood cell parameters [16].
Methods
Ethics statement
The study has been conducted according to the recommendations of the Declaration of Helsinki. The study protocol of SHIP was approved by the medical ethics committee of the University of Greifswald. Written informed consent was obtained from each of the study participants.
Study design
Initially, EDTA-plasma samples from 384 participants were randomly selected from the SHIP-TREND cohort. Study design and sampling methods for SHIP-TREND were previously described [16]. Briefly, SHIP-TREND is a longitudinal population-based cohort study assessing the prevalence and incidence of common diseases and their risk factors. Study participants were randomly selected from the population registries in North- and East-Pomerania.
The laboratory workflow for RT-qPCR based miRNA analysis using the Serum/Plasma Focus microRNA PCR Panel V3.M (Exiqon A/S, Vedbaek, Denmark) involved several quality control steps which resulted in the exclusion of 12 plasma samples. The descriptive statistics of the remaining study participants are provided in Table 1. Blood cell parameters were measured on an automated haematology system (XT 200 or XE 5000, Sysmex, Europe).
Table 1.
Sex | Age (years) | BMI (kg/m2) | |||
---|---|---|---|---|---|
number | Mean ± SD | range | Mean ± SD | range | |
male | 187 | 49.3 ± 14.5 | 22-79 | 27.6 ± 3.9 | 17.7-39.0 |
female | 185 | 50.2 ± 13 | 22-79 | 27.4 ± 5.0 | 18.7-48.1 |
total | 372 | 49.7 ± 13.8 | 22-79 | 27.5 ± 4.4 | 17.7-48.1 |
Preparation of plasma miRNAs
Non-cellular blood circulating miRNAs were isolated from 200 μl plasma using the miRCURY™ RNA Isolation Kit –Biofluids (Exiqon A/S) according to the manufacturer’s instructions. To ensure high and reproducible RNA yield from EDTA-plasma samples, bacteriophage MS2 carrier RNA was added to each sample during the purification procedure. Reverse transcription reactions were performed using Universal cDNA Synthesis Kit II (Exiqon A/S) according to the manufacturer’s instructions. Before using RNA samples for miRNA profiling, the yield of typical plasma miRNAs, absence of PCR inhibitors as well as of haemolysis in the samples was assessed by use of a microRNA QC PCR Panel (Exiqon A/S).
Profiling of plasma miRNAs
Exiqon Serum/Plasma Focus microRNA PCR Panels, 384 well (V3.M) were used in a RT-qPCR approach to determine the plasma levels of 179 human miRNAs. The qPCR was performed using a 7900 HT Real-time PCR system (Applied Biosystems, Carlsbad, CA, USA) with 42 amplification cycles employing the cycling parameters recommended by Exiqon. Raw data were processed using SDS 2.4 (Applied Biosystems) to assign the baseline and threshold for Ct (threshold cycle: the PCR cycle at which the target is quantified in a given sample, according to Real-time PCR Data Markup Language (RDML) guidelines [17]) determination. To determine the technical variation between the Exiqon Serum/Plasma Focus microRNA PCR Panel plates, the inter-plate calibrator (IPC) (UniSp3) was analysed. Ct values of the IPC were 20 ± 0.2 (mean ± SD) across all samples, and thus highly similar.
Computational analyses
All computational analyses were implemented in R (3.1.2 “Pumpkin Helmet”) [18]. The code is available upon request. Generally, a miRNA-wise two-step regression procedure was employed. Through the evaluation of a first regression model the data were corrected for technical influences (see Regressing-out of technical parameters). The second step comprised the assessment of associations between miRNAs and phenotypes in a separate regression model (see Analysis of associations between miRNA levels and phenotypes).
Data pre-processing
We ran the RT-qPCR for 42 cycles and specified the detection cut off according to manufacturer’s recommendation [15]. The Ct value threshold established in [15] for the very sensitive Exiqon platform has already been successfully employed in other studies on low-abundant miRNAs [19, 20]. Thus, also in our study Ct values below 37 were considered for quantification and Ct values above 37 were treated as missing because they were considered to be too close to the detection limit of the assay. Remaining Ct values were normalized to the lower quartile per sample. That is, per sample the lower quartile across all Ct values, excluding spike-ins, was subtracted from each individual sample Ct value, yielding ∆Ct values (small ∆Ct values indicate high miRNA levels). Only miRNAs with at least 100 valid (i.e. non-missing) ∆Ct values and normal ∆Ct value distribution across all samples were kept. Thus, all association analyses are based on a set of 155 miRNAs that satisfied these criteria.
Regressing-out of technical parameters
Plasma miRNA data were influenced by a number of technical parameters. Among these were the storage time of plasma samples in the biobank ranging from 1035 to 1774 days (dt_biobank) and the Ct values of synthetic spiked-in miRNAs monitoring the efficiency of miRNA extraction (UniSp2 and the difference between Ct values of UniSp4 and UniSp2). Before further analyses, these parameters were regressed out of the data. To that end, linear regression according to the model ∆Ct ~ dt_biobank + UniSp2 + UniSp4-UniSp2 , which treats the ∆Ct values as dependent variables and the technical parameters as independent variables was performed for each miRNA. The resulting residuals represent the variance in miRNA levels that cannot be explained by the aforementioned technical parameters. These residuals were used as dependent variables in later models to detect associations between miRNAs and phenotypes.
Analysis of associations between miRNA levels and phenotypes
To identify associations between plasma miRNA levels and the phenotypes investigated in this study, linear regression models were fitted for each miRNA separately. These models contained the residuals of the model for technical adjustment (see Regressing-out of technical parameters) as dependent variables. That is, the goal of these models was to explain the variance in miRNA levels not due to technical parameters. As independent variables the phenotype(s) examined or adjusted for (i.e. age, BMI, sex), as well as important blood cell parameters (BCPs) (see Identification of blood cell parameters) were used. The strength of a miRNA-phenotype association was assessed by the Benjamini-Hochberg-corrected p-value (q-value) of the corresponding model coefficient.
Identification of blood cell parameters
An elastic net regularized regression model [21] was employed to identify important BCPs that affect miRNA levels. The motivation to identify BCPs via an elastic net was two-fold. First, the elastic net selects the smallest subset of independent variables most accurately predicting the dependant variable. This results in the incorporation of as few BCPs into our models as possible, while accounting for as much variation in the miRNA data as possible. Second, the elastic net accounts for correlation between covariates. This is important here, since many BCPs are inter-correlated. The elastic-net regularized linear regression models were evaluated through a leave-one-out cross-validation as implemented in the R package glmnet (v 1.9-8) [22]. These models comprised ∆Ct values as dependent variables and technical parameters and BCPs as independent variables (for a list of all BCPs, see Additional file 1: Table S1). Alpha for these models was set to 0.5 to balance-out the L1 and L2 penalties. BCPs frequently selected by the elastic net across all miRNAs were incorporated into linear regression models assessing miRNA – phenotype associations. These BCPs were haematocrit, platelet count, and mean platelet volume. A Manhattan plot of these BCPs in the linear model is provided as Additional file 1: Figure S1.
Results
For the present study, data from 187 men and 185 women were used. Age of the participants varied between 22 and 79 years and the body mass index varied between 17.7 and 48.1 (kg/m2) (Table 1).
Association of plasma miRNA levels with age, BMI, and sex
For the present proof-of-principle study, we investigated associations between plasma miRNA levels and the phenotypes BMI, sex, and age (Fig. 1).
The linear regression models incorporated all three phenotypes. Significant (q < 0.05) associations with age were detected for seven miRNAs. The strongest were observed for hsa-miR-126-3p and hsa-miR-21-5p (q < 0.001) (Fig. 2a, and Additional file 2: Table S2). Altogether 15 miRNAs were significantly associated with BMI. Here, the most significant associations were observed for hsa-miR-122-5p, hsa-miR-148a-3p and hsa-miR-505-3p (q < 0.001) (Fig. 2a and Additional file 3: Table S3). Regarding sex, 35 miRNAs were found to be significantly associated (Fig. 2a and Additional file 4: Table S4). Among these, several miRNAs such as hsa-miR-145-5p, hsa-miR-451a, hsa-miR-143-3p, hsa-miR-16-2-3p are known to originate from blood cells and to be involved in haematopoiesis.
The number of miRNAs associated to multiple phenotypes was strikingly small (Fig. 3). Only hsa-miR-93-5p was associated with both age and BMI. Also the overlap between age and sex was restricted to only one miRNA, namely hsa-miR-142-3p. The miRNAs hsa-miR-143-3p, hsa-145-5p, and hsa- miR-148a-3p were associated with both sex and BMI. There was no miRNA associated with all three phenotypes.
Modified associations after adjustment for blood cell parameters
Additional adjustment was performed using appropriate blood cell parameters (BCPs, see Methods section for details). The number of significantly (q < 0.05) age-associated miRNAs rose to 12 after adjustment for sex, BMI, and BCPs, 7 of which overlapped with the previous results (Fig. 2b, Additional file 2: Table S2). The strongest associations with age were observed for hsa-miR-126-3p, hsa-miR-30c-5p, and hsa-miR-142-3p (q < 0.001) (Fig. 2b, Additional file 2: Table S2). However, the effect sizes (β∆Ct from linear regression) of associations with age were quite small (0.01 to -0.01). Adjustment for age, sex, and BCPs resulted in the identification of 19 significantly BMI-associated miRNAs, 15 of which overlapped with the previous results (Fig. 2b, Additional file 3: Table S3). The most significant associations with BMI were still observed for hsa-miR-122-5p, hsa-miR-148a-3p and hsa-miR-505-3p (q < 0.001).
Adjustment for age, BMI, and BCPs reduced the number of significantly sex-associated miRNAs from 36 to 7 (Fig. 2b, Additional file 4: Table S4). The association strength of the selected BCPs (haematocrit, platelet count, and mean platelet volume) is shown in the Manhattan plot in Additional file 1: Figure S1. Nevertheless, remaining associations were still accompanied by profound effect sizes (β∆Ct = 0.33 to –0.35). The most significant associations with sex were observed for hsa-miR-145-5p, hsa-miR-150-5p and hsa-miR-142-3p (q < 0.01).
The overlap of association of miRNAs with different phenotypes after the adjustment for the respective other two phenotypes and BCPs was also investigated. In the fully adjusted models, only few miRNAs were significantly associated with more than one phenotype (Fig. 4): hsa-miR-93-5p with both BMI and age, hsa-miR-148a-3p and hsa-miR-145-5p with both BMI and sex, and hsa-miR-142-3p with both age and sex. Again, none of the miRNAs was associated with all three phenotypes.
Discussion
In the last few years, the interest in non-cellular blood circulating miRNAs (plasma miRNAs) as biomarkers present in easily accessible body fluids increased continuously. Various studies analysed associations between plasma miRNAs and specific disease phenotypes, mostly using a case-control design [11]. However, these studies were frequently limited by relatively small sample sizes as well as a number of biases, e.g. the lack of appropriate adjustment for confounding factors such as age [11]. So far a limited number of large population-based phenotype-miRNA association studies have been performed [8–11]. Furthermore, while whole blood is indeed easily accessible for sampling, its composition is complex. Different cell types and tissues in contact with blood might contribute miRNA species to the plasma miRNA pool in different proportions. Without appropriate adjustment, plasma miRNA profiles will always partially reflect the individual blood composition at the sampling time [23, 24]. Thus, in the context of the search for highly informative biomarkers, it appears reasonable to focus on miRNAs that are not or only marginally affected by the BCPs.
In the present study, we quantified plasma miRNA levels of 372 individuals from the population-based SHIP-TREND cohort and analysed the associations of these miRNA profiles with age, BMI, and sex under consideration of the BCPs. The numbers of age-associated and BMI-associated miRNAs were similar. A positive age-correlation was found for hsa-miR-126-3p, thereby confirming a recently published study [25]. Further miRNAs detected to be associated with age in this study such as hsa-miR-30, hsa-miR-93, hsa-miR-21 and hsa-miR-142-3p were also previously reported as age-related [14, 26, 27]. However, hsa-miR-17, hsa-miR-19b, hsa-miR20a and hsa-miR-106a could not be validated as age-associated plasma miRNAs in our population based study [28]. Further miRNAs such as hsa-miR-26a-5p, hsa-let-7a-5p, hsa-miR-101-3p and hsa-miR-23b-3p were found to be age associated but have not yet been described. However, in all cases, the effect sizes of the age-miRNA-associations were rather small, indicating a less pronounced relationship between age and plasma miRNA levels, as compared to, e.g., BMI-miRNA-associations.
Several plasma miRNAs were significantly associated with BMI in the present study. One of the most prominent was hsa-miR-122-5p which is highly abundant in the adult liver [29] where it acts as a key regulator of cholesterol and fatty-acid metabolism [30]. This miRNA was recently described as a serum biomarker for liver injury in chronic hepatitis B and C, non-alcoholic fatty liver disease (NAFLD), and drug-induced liver disease [31–34]. Consistently, the comparison of miRNAs known to be synthesized in large amounts in adult human liver [35] with the significantly BMI-associated plasma miRNAs detected in this study revealed an overlap of 12 miRNAs (hsa-miR-99a, hsa-miR-194, hsa-miR-143, hsa-miR-93, hsa-miR-185, hsa-miR-885, hsa-miR-193b, hsa-miR-145, hsa-miR-19b, hsa-miR-18a, hsa-miR-486, and hsa-miR-148a). The prominent BMI-associated miRNAs belong to different families organized in clusters such as miR-106b ~ 25 (hsa-miR-93), miR-106a ~ 363 (hsa-miR-106a) and miR-17 ~ 92 (hsa-miR-18a, hsa-miR-20a and hsa-miR-19b-1). The obvious high portion of liver-specific miRNAs whose blood levels were found to be positively correlated with BMI points towards release of these miRNAs from lysing hepatocytes into the circulation as a consequence of subclinical or/ and manifest NAFLD which is in turn strongly positively associated with an increased BMI.
A recently published microarray-based study on the associations between peripheral blood circulating miRNAs with age as well as sex revealed only a limited association between sex and miRNA patterns [14]. In the present study, we also investigated the association between sex and plasma miRNA profile. Before adjustment for BCPs there were more miRNAs significantly associated with sex than with age or BMI. However, a high proportion of these sex-associated miRNAs most probably originates from blood cells. Monocytes, thrombocytes, granulocytes, lymphocytes, reticulocytes and erythrocytes all contain several cell type specific as well as ubiquitously expressed miRNAs in varying amounts [24, 36]. The total blood cell mass in the circulation of women is generally smaller compared to men. This was confirmed for multi-ethnic populations [37] and is reflected in a 12 % lower mean haemoglobin level in female venous blood compared to men [38] as well as in lower haematocrit values. Consistently, in the present study, besides significantly elevated erythrocyte counts in men compared with women (Additional file 1: Table S1), erythrocyte-specific miRNAs such as hsa-miR-451a or hsa-miR-16-2-3p exhibited higher levels in men, which is also in line with the previously published observation that plasma miRNAs correlate to blood cell counts [24]. As expected, the sex-associated signals for blood-cell-specific miRNAs largely vanished after adjustment for BCPs in the present study.
Regulatory roles in haematopoiesis were described for hsa-miR-451 and hsa-miR-16. These are involved in the differentiation of erythroid progenitor cells into red blood cells. Similarly, hsa-miR-150 activates the differentiation of common lymphoid progenitors into T cells, B cells and natural killer cells [39]. As potential sources of such miRNAs, lymphoid cells such as T cells, B cells (hsa-miR-150, hsa-miR-142), platelets (hsa-miR-142) and monocytes (hsa-miR-145) have been mentioned [24, 40]. In our study this is reflected by, e.g. significantly increased platelet levels in women compared to men (Additional file 1: Table S1). Recently, it was hypothesized that differential expression of miRNAs in male and female immune cells contributes to sex differences in immune capabilities and susceptibilities to autoimmune diseases [41].
Hence, in studies associating plasma miRNA levels with specific clinical phenotypes, special attention should be paid to sex differences and BCPs.
It is clear that further increasing the sample size might reveal additional associations that until now did not pass the significance threshold. Furthermore, while the RT-qPCR approach based on Exiqon´s Serum/Plasma Focus Panels V3 offers a high specificity and sensitivity on measured miRNAs in a high throughput manner, it is limited with respect to the number of detectable miRNAs [15]. Nevertheless, our results corroborate the general feasibility of association studies with plasma miRNAs.
Conclusions
In the present association study we demonstrate that plasma miRNA profiles based on a population-based study cohort reflect individual sex, age, and BMI. Therefore, our findings underline the importance of considering these phenotypes as potential covariates in such studies. The established experimental and computational workflow presented here will be used in future screening studies for associations with disease-specific phenotype parameters. Beyond that, replication of our primary association findings in further independent cohorts is intended.
Acknowledgments
The authors thank Ulrike Lissner for excellent work in context of RNA preparation, quality control and RT-qPCR measurements.
Funding
SHIP is part of the Community Medicine Research net of the University of Greifswald, Germany, which is funded by the Federal Ministry of Education and Research (BMBF, grants no. 01ZZ9603, 01ZZ0103 and 01ZZ0403), the Ministry of Cultural Affairs and the Social Ministry of the Federal State of Mecklenburg-West Pomerania. Furthermore, the study was funded by the BMBF through a grant for the Greifswald Approach to Individualized Medicine (GANI_MED, 03IS2061A).
Abbreviations
- BCP
Blood cell parameters
- BH
Benjamini-Hochberg
- BMI
Body mass index
- miRNA
microRNA
- NAFLD
Non-alcoholic fatty liver disease
- RT-qPCR
Reverse transcription-quantitative PCR
- SHIP-TREND
Study of Health in Pomerania-Trend
Additional files
Footnotes
Sabine Ameling, Tim Kacprowski and Ravi Kumar Chilukoti contributed equally to this work.
Competing interests
The authors declare that they have no competing interests.
Authors’ contributions
SA contributed to the study design, data evaluation, analysis and interpretation of data and wrote the manuscript. TK contributed to data evaluation, designed computational analyses and wrote the manuscript. RKC extracted miRNA of plasma samples, performed RT-qPCR analysis and data collection. CM, VL, KS and MP contributed to computational analysis. GH contributed to study design, data interpretation and wrote the manuscript. NF contributed to sample collection. EH contributed to the design of the study, data analysis and preparation of the manuscript. UV initiated the study and contributed to the study design, data evaluation and writing of the manuscript. All authors read and approved the final manuscript.
Authors’information
Not applicable.
Contributor Information
Sabine Ameling, Email: sabine.ameling@uni-greifswald.de.
Tim Kacprowski, Email: tim.kacprowski@uni-greifswald.de.
Ravi Kumar Chilukoti, Email: ravikumar.ch@gmail.com.
Carolin Malsch, Email: carolin_malsch@live.de.
Volkmar Liebscher, Email: volkmar.liebscher@uni-greifswald.de.
Karsten Suhre, Email: karsten@suhre.fr.
Maik Pietzner, Email: maik.pietzner@uni-greifswald.de.
Nele Friedrich, Email: nele.friedrich@uni-greifswald.de.
Georg Homuth, Email: georg.homuth@uni-greifswald.de.
Elke Hammer, Email: hammer@uni-greifswald.de.
Uwe Völker, Phone: +49-3834-865870, Email: voelker@uni-greifswald.de.
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