Hindawi Publishing Corporation Disease Markers Volume 2015, Article ID 351015, 5 pages http://dx.doi.org/10.1155/2015/351015
Research Article Analysis of Serum MicroRNAs as Potential Biomarker in Coronary Bifurcation Lesion Yan Liu, Shaoliang Chen, Junjie Zhang, Shoujie Shan, Liang Chen, Rong Wang, Jing Kan, and Tian Xu Department of Cardiology, Nanjing First Hospital, Nanjing Medical University, Changle Road No. 68, Nanjing, Jiangsu 210029, China Correspondence should be addressed to Shaoliang Chen; [email protected] Received 31 October 2014; Revised 11 January 2015; Accepted 17 February 2015 Academic Editor: Varodom Charoensawan Copyright © 2015 Yan Liu et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. Recent evidence suggests that cell-derived circulating miRNAs may serve as the biomarkers of cardiovascular diseases. However, no study has investigated the potential of circulating miRNAs as biomarker for coronary bifurcation lesion. In this study, we aimed to characterize the miRNA profiles that could distinguish coronary bifurcation lesion and identify potential miRNAs as biomarkers of coronary bifurcation lesion. We employed miRNA microarray to screen serum miRNAs profiles of patients with coronary bifurcation lesion and coronary nonbifurcation lesions. We identified 197 miRNAs differentially expressed, including 150 miRNAs upregulated and 47 miRNAs downregulated. We chose 3 miRNAs with significant differences for further testing in 200 patients. RT-PCR analysis of serum samples confirmed that miR30d was upregulated and miR1246 was downregulated in the serum of coronary bifurcation lesion patients compared with nonbifurcation lesion patients. Our findings suggest that these miRNAs may have a role in the pathogenesis of coronary bifurcation lesion and may represent novel biomarkers for the diagnosis and prognosis of coronary bifurcation lesion.
1. Introduction
2. Methods
Coronary artery disease (CAD) is one of the leading causes of death worldwide. The pathogenesis of CAD remains incompletely understood and both genetic and environmental factors are involved in this complex disease [1, 2]. Coronary bifurcation lesion is the most challenging lesion in percutaneous coronary interventional medicine because the rate of restenosis and major adverse cardiac event is significantly higher than nonbifurcation lesion [3]. MicroRNAs (miRNAs) are key regulators of gene expression that have been widely associated with a variety of diseases [4, 5]. Recent evidence suggests that cell-derived circulating miRNAs may serve as the biomarkers of cardiovascular diseases including CAD [6]. However, no study has investigated the potential of circulating miRNAs as biomarker for coronary bifurcation lesion. In this study, we aimed to characterize the miRNA profiles that could distinguish coronary bifurcation lesion and identify potential miRNAs as biomarkers of coronary bifurcation lesion.
2.1. Patients. In the matched case-control study, we recruited 5 patients with coronary bifurcation lesion aged 45–87 years (average 72.4 ± 16.4 years) and 5 control patients with coronary nonbifurcation lesion aged 46–75 years (average 59.6 ± 11.7 years). For large sample validation, we recruited 100 patients with coronary bifurcation lesion aged 45–88 years (average 67.8±10.9 years) and 100 control patients with coronary nonbifurcation lesion aged 40–84 years (average 65.5 ± 10.2 years). Serum samples of all subjects were collected. Coronary bifurcation lesion was defined as a junction of a main vessel and a side branch (with a minimal diameter of 1.5 mm) [7]. Coronary bifurcation lesion patients and control subjects had no other concomitant diseases, including severe cardiomyopathy or valvular heart disease, lung disease, significant cardiac dysfunction or liver and kidney dysfunction, thrombotic disease or blood disease, and connective tissue disease or malignancy or active infection such as hepatitis and tuberculosis.
2 2.2. Serum Samples. The blood was collected from each subject into EDTA anticoagulant tube and centrifuged at 3,000 rpm for 10 min, and the supernatant was stored at −80∘ C. 2.3. RNA Extraction. Total RNA was isolated using TRIzol (Invitrogen) and miRNeasy Mini Kit (QIAGEN) according to the manufacturer’s instructions. RNA was dissolved in nuclease-free water by passing a few times through a pipette tip. RNA quality and quantity were measured by using nanodrop spectrophotometer (ND-1000, Nanodrop Technologies) and RNA integrity was determined by gel electrophoresis. 2.4. RNA Labeling. RNA was labeled using miRCURY Hy3/Hy5 Power Labeling Kit (Exiqon, Vedbaek, Denmark) according to the manufacturer’s guideline. One microgram of each sample was 3 -end-labeled with Hy3TM fluorescent label, using T4 RNA ligase. The mixture was incubated for 30 min at 37∘ C, and the reaction was terminated by incubation for 5 min at 95∘ C. Then, 3.0 𝜇L of labeling buffer, 1.5 𝜇L of fluorescent label (Hy3TM), 2.0 𝜇L of DMSO, and 2.0 𝜇L of labeling enzyme were added into the mixture. The labeling mixture was incubated for 1 h at 16∘ C, and the reaction was terminated by incubation for 15 min at 65∘ C.
Disease Markers Table 1: The characteristics of the patients for microarray analysis.
Age (years) Males Hypertension Diabetes Stroke Current smoker Lesion site LAD Lesion site LM Lesion site RCA Lesion calcification Needing rotablation Restenosis Thrombus TIMI grade 0 TIMI grade 1 Medina classification 111
Coronary bifurcation lesion 𝑛=5
Coronary nonbifurcation lesion 𝑛=5
72.4 ± 16.4 4 (80%) 4 (80%) 0 (0%) 2 (40%) 2 (40%) 4 (80%) 0 (0%) 1 (20%) 0 (0%) 0 (0%) 0 (0%) 1 (20%) 3 (60%) 2 (40%) 0 (0%)
59.6 ± 11.7 2 (40%) 4 (80%) 0 (0%) 2 (40%) 2 (40%) 1 (20%) 4 (80%) 0 (0%) 3 (60%) 1 (20%) 1 (20%) 1 (20%) 2 (40%) 3 (60%) 4 (80%)
2.5. miRNA Microarray. Hy3TM-labeled samples were hybridized on the miRCURYTM LNA Array (v.18.0) (Exiqon) according to the manufacturer’s manual. Following the hybridization, the slides were achieved, washed several times using Wash Buffer Kit (Exiqon), and finally dried by centrifugation for 5 min at 400 rpm. Then, the slides were scanned using the Agilent Microarray Scanner (part number G2505C).
Unsupervised hierarchical clustering and correlation analysis was performed on miRNA data. Data were expressed as mean ± SD and analyzed using SPSS13.0 software. Categorical variables were compared by 𝜒2 test, and continuous variables were compared by 𝑡-test. A value of 𝑃 < 0.05 was considered significant.
2.6. Quantitative RT-PCR. Quantitative PCR was performed on an ABI 7500 system (Applied Biosystems, Foster City, CA). RNA was reverse transcribed with the TaqMan miRNA Reverse Transcription Kit (ABI) according to the manufacturer’s instructions. Subsequently, 2.5 ul of the product was used for detecting miRNA expression by quantitative polymerase chain reaction with TaqMan miRNA Assay Kits (ABI).
3.1. The Characteristics of the Patients. To characterize the miRNAs profiles of coronary bifurcation lesion, we recruited 5 patients with coronary bifurcation lesion and 5 patients with coronary nonbifurcation lesion as the control. The characteristics of these patients were listed in Table 1.
2.7. Data Analysis. The intensity of green signal was calculated after background subtraction and four replicated spots of each probe on the same slide have been averaged. We used Median Normalization Method to obtain “Normalized Data,” Normalized Data = (Foreground − Background)/median; the median was 50 percent quantile of microRNA intensity which was larger than 30 in all samples after background correction. After normalization, the statistical significance of differentially expressed miRNA was analyzed by 𝑡-test. A threshold cut-off value was set to 1 fold change which indicates that the expression of a given miRNA is uniform in both case and control groups. The fold change of greater than 1 indicated upregulated miRNAs, whereas the fold change of less than 1 indicated downregulated miRNAs.
3. Results
3.2. Identification of miRNAs Expression Patterns of Patients with Coronary Bifurcation Lesion. We performed microarray analysis to identify miRNAs expression patterns of patients with coronary bifurcation lesion. We made a heat map to visualize the results of the two-way hierarchical clustering of miRNAs (Figure 1). The color scale shown at the top illustrated the relative expression level of a miRNA: red represented a high relative expression level while green represented a low relative expression level [8]. Furthermore, we made a Volcano plot to illustrate miRNAs differentially expressed between coronary bifurcation lesion and coronary nonbifurcation lesion (Figure 2). We identified 197 miRNAs differentially expressed between coronary bifurcation lesion and coronary nonbifurcation lesion, including 150 miRNAs upregulated and 47 miRNAs downregulated (Supplemental File 1 in Supplementary Material available online at http://dx.doi.org/10.1155/2015/351015).
3 Table 2: Confirmation of differential miRNA expression in 200 patients.
71_exp
1_exp
41_exp
9_exp
42_exp
38_ctl
58_ctl
60_ctl
67_ctl
hsa-miR-4288 hsa-miR-4500 hsa-miR-3184-3p hsa-miR-3664-5p hsa-miR-30d-5p hsa-miR-877-5p hsa-miR-4297 hsa-miR-99b-5p hsa-miR-3920 hsa-miR-222-3p hsa-miR-584-5p hsa-miR-4768-5p hsa-miR-130b-5p hsa-miR-4654 hsa-let-7d-3p hsa-miR-151a-3p hsa-miR-423-3p hsa-miR-155-5p hsa-miR-221-3p hsa-miR-4483 hsa-miR-146b -5p hsa-miR-382-5p hsa-miR-4709-3p hsa-miR-3156-3p hsa-miR-3976 hsa-miR-4456 hsa-miR-5681b hsa-miR-664b-3p hsa-miR-4726-5p hsa-miR-3941 hsa-miR-3686 hsa-miR-4531 hsa-miR-4644 hsa-miR-3611 hsa-miR-1246 hsa-miR-501-3p hsa-miR-937-3p hsa-miR-33b-5p hsa-miR-409-3p ebv-miR-BART17-5p hsa-miR-5582-3p hsa-miR-3605-3p hsa-miR-339-5p hsa-miR-103b hsa-miR-504 hsa-miR-190b hsa-miR-671-3p hsa-miR-652-3p hsa-miR-4667-3p hsa-miR-5195-5p hsa-miR-181d hsa-miR-146a-5p hsa-miR-432-5p hsa-miR-654-3p kshv-miR-K12-3-5p hsa-miR-92b-3p hsa-miR-2115-3p hsa-miR-1266 hsa-miR-3183 hsa-miR-30e-3p hsa-miR-4306 hsa-miR-1255a hsa-miR-3171 hsa-miR-1304-5p sv40-miR-S1-5p hsa-miR-4777-5p kshv-miR-K12-5-5p hsa-miR-5002-5p hsa-miR-630 hsa-miR-1273e hsa-miR-5006-3p hsa-miR-4780 hsa-miR-498 hsa-miR-4725-5p hsa-miR-4472 hsa-miR-4478 hsa-miR-523-5p hsa-miR-522-5p hsa-miR-519c-5p hsa-miR-519b-5p hsa-miR-519a-5p hsa-miR-518e-5p hsa-miR-576-5p hsa-miR-1264 hsa-miR-3680-5p hsa-miR-1285-5p hsa-miR-4784 hsa-miR-204-3p hsv1-miR-H5-3p hsa-miR-520a-5p hsa-miR-4459 hsa-miR-4521 hsa-miR-5007-3p hsa-miR-548an hsa-let-7a-2-3p hsa-miR-5581-3p hsa-miR-3940-5p hsa-miR-574-3p hsa-miR-3938 hsa-miR-4795-5p hsa-miR-4326 hsa-miR-22-5p hsa-miR-4451 hsa-miR-1587 hsa-miR-3146 hsa-miR-4800-5p hsa-miR-3158-5p hsa-miR-4682 hsa-miR-4712-3p hsa-miR-4419b hsa-miR-3935 hsa-miR-4762-5p hsa-miR-1273g-3p hsa-miR-665 hsa-miR-506-5p hsa-miR-1255b-2-3p hsa-miR-548t-3p hsa-miR-548ap-3p hsa-miR-548aa hsa-miR-214-3p hsa-miR-5684 hsa-miR-5197-5p hsa-miR-1972 hsa-miR-761 hsa-miR-125b-2-3p hsa-miR-4694-5p hsa-miR-4503 hsa-miR-3915 hsa-miR-298 hsa-miR-3688-5p hsa-miR-647 hsa-miR-4661-5p hsa-miR-421 hsa-miR-3126-5p hsa-miR-3145-5p hsa-miR-3673 hsa-miR-4254 hsa-miR-5006-5p hsa-miR-767-5p hcmv-miR-UL22A-3p hsa-miR-148b-5p hsa-miR-2115-5p hsa-miR-1272 hsa-miR-4756-5p hsa-miR-4723-5p hsa-miR-3119 hsa-miR-4299 hsa-miR-708-5p hcmv-miR-US25-2-5p hsa-miR-4716-3p hsa-miR-764 hsa-miR-527 hsa-miR-518a-5p hsa-miR-3654 hsa-miR-1255b-5p hsa-miR-3123 hsa-miR-2392 hsa-miR-375 hsa-miR-3160-5p hsa-miR-635 hsa-miR-890 hsa-miR-4445-3p hsa-miR-5698 hsa-miR-4468 hsa-miR-7-2-3p hsa-miR-23c hsa-miR-3911 hsa-miR-620 hsa-miR-192-5p hsa-miR-1204 hsa-miR-3126-3p hsa-miR-20b-3p hsa-miR-3135a hsa-miR-920 hsa-miR-4447 kshv-miR-K12-1-3p hsa-miR-2964a-5p hsa-miR-5002-3p hsa-miR-891a hsa-miR-2681-5p hsa-miR-490-3p hsa-miR-4477a hsa-miR-4275 hsa-miR-500a-5p hsa-miR-622 hsv1-miR-H8-5p hsa-miR-422a hsa-miR-5196-3p hsa-miR-938 hsa-miR-4300 hsa-miR-516b-5p hsa-miR-15a-3p hsa-miR-3926 hsa-miR-516b-3p hsa-miR-516a-3p hsa-miR-424-5p hsa-miR-4305 hsa-miR-3689e hsa-miR-3689b-5p hsa-miR-3689a-5p hsa-miR-4307 hsa-miR-3649 kshv-miR-K12-5-3p hsa-miR-548e hsa-miR-4273 hsa-miR-589-5p hcmv-miR-UL36-5p
Figure 1: Heat map illustrating the expression patterns of upregulated and downregulated miRNAs in patients with bifurcation lesion. Upregulated miRNAs were indicated by red while downregulated miRNAs were indicated by green. The three candidate miRNA markers miR30d, miR222, and miR1246 were underlined in red.
Age (years) Males Smoker Hypertension Diabetes miR30d level miR222 level miR1246 level
Bifurcation lesion (𝑛 = 100)
Nonbifurcation lesion (𝑛 = 100)
𝑃
67.8 ± 10.9 52 52 61 28 0.0258 ± 0.0566 0.1024 ± 0.0616 0.0346 ± 0.0567
65.5 ± 10.2 56 50 60 30 0.0017 ± 0.0006 0.0953 ± 0.0693 0.3004 ± 0.2469
0.377 0.55 0.82 0.76 0.51 0.000 0.881 0.000
Volcano plot (exp. versus ctl.)
6 5
−Log10 (P value)
Color key and histogram 80 40 0 −5 0 5 Value
53_ctl
Count
Disease Markers
4 3 2 1 0 −4
−2
0 2 Log2 fold change
4
Figure 2: miRNAs differentially expressed in patients with bifurcation lesion and patients with nonbifurcation lesion. The volcano plots illustrated miRNAs differentially expressed: dots in black indicted the miRNAs that did not reach significant changes of expression; dots in red on the left indicated the miRNAs that had significant downregulation of expression; and dots in red on the right indicated the miRNAs that had significant upregulation of expression.
3.3. Confirmation of Different miRNAs in Serum of Patients with Coronary Bifurcation Lesion. To confirm our results, we chose three of the most differentially expressed miRNAs, including 2 upregulated (miR30d and miR222) and one downregulated (miR1246), which showed difference by more than 10 times. We enrolled 100 patients with bifurcation lesion and 100 patients with nonbifurcation lesion. As illustrated in Table 2, there were no significant differences in the two groups, including the age, the gender, the status of smoking, hypertension, and diabetes. As shown in Figure 3, RT-PCR analysis showed that circulating serum level of miR30d was profoundly elevated in patients with coronary bifurcation lesion compared to nonbifurcation lesion patients (𝑃 < 0.05). Circulating level of
4
Disease Markers
20000 15000 10000
hsa-miR-4297
hsa-miR-222-3p
hsa-miR-4288
hsa-miR-30d-5p
hsa-miR-423-3p
hsa-miR-2115-3p
hsa-miR-1246
hsa-miR-4644
hsa-miR-3976
0
hsa-miR-3611
5000 hsa-miR-4306
Relative level
25000
Case Control
Figure 3: qRT-PCR analysis of several miRNAs differentially expressed in case and control groups. Case: bifurcation lesion patients; control: nonbifurcation lesion patients. Shown were representative data from three independent experiments.
miR222 was modestly but not significantly increased in coronary bifurcation lesion patients compared to nonbifurcation lesion patients (𝑃 = 0.881). Moreover, serum level of miR1246 was significantly lower in bifurcation lesion patients than in nonbifurcation lesion patients (𝑃 < 0.05). These data confirmed our results of microarray analysis.
4. Discussion Coronary artery disease (CAD) is a multifactorial disease that can be influenced by a multitude of environmental and heritable risk factors. CAD has serious impact on human life and health. Coronary atherosclerosis is a main reason that causes CAD. Atherosclerosis is a chronic and progressive pathologic process characterized by the accumulation of lipid and fibrous elements in the large arteries, which causes a number of cardiovascular-related diseases. The development of atherosclerosis involves the following steps: foam cell formation, fatty streak accumulation, migration and proliferation of vascular smooth muscle cells (VSMCs), and fibrous cap formation. Finally, the rupture of the unstable fibrous cap causes thrombosis that leads to unstable coronary syndromes, myocardial infarction, and stroke. Coronary intervention is an effective means of coronary heart disease treatment. Coronary bifurcation is prone to develop atherosclerotic plaque due to turbulent blood flow and high shear stress. Treatment of coronary bifurcation lesion represents a challenging area in interventional cardiology but recent advances in percutaneous coronary interventions (PCI) have led to the dramatic increase in the number of patients successfully treated percutaneously. Compared with nonbifurcation interventions, bifurcation interventions have a lower rate of procedural success, higher procedural costs, longer hospitalization, and a higher clinical and angiographic restenosis. Introduction of drug-eluting stents (DES) has resulted in a lower event rate and reduction of main vessel
(MV) restenosis. However, side branch (SB) ostial residual stenosis and long-term restenosis remain a problem [9]. MicroRNAs (miRNAs) are a class of short, noncoding, single stranded RNA molecules, approximately 22 nucleotides in length. They negatively regulate gene expression either through inhibition of mRNA translation or by promoting mRNA degradation. Emerging evidence suggests that miRNAs are pivotal regulators of various processes including cell proliferation, differentiation, apoptosis, survival, motility, and morphogenesis [10]. Recently, specific miRNA expression profiles have been reported as a prognostic factor or a predictive factor for disease progression. In particular, serum miRNAs may be used as a biomarker in diagnosis [6]. In pathological process, miRNAs are linked to myocardial hypertrophy, myocardial fibrosis, heart failure, and arrhythmias. A series of miRNAs are involved in pathological progression of coronary heart disease and play pivotal roles in the development of the disease [11–13]. Hoekstra et al. investigated the potential of miRNAs as biomarkers for CAD and reported that unstable angina pectoris patients could be discriminated from stable patients based on the relatively high expression levels of miR-134, miR-198, and miR-370 in peripheral blood mononuclear cells [14]. Therefore, we hypothesized that in CAD serum miRNA levels could be changed and those miRNAs can be used as the biomarkers. In this study, we performed microarray analysis to identify 197 miRNAs differentially expressed in the serum of patients with coronary bifurcation lesion, including 150 miRNAs upregulated and 47 miRNAs downregulated. After a rigorous selection, we screened 3 miRNAs differentially expressed, including downregulated miR1246 and upregulated miR30d and miR222. Further large sample validation in 200 patients demonstrated a distinct serum miRNA expression pattern in patients with coronary bifurcation lesion; miR30d was upregulated and miR1246 was downregulated compared with nonbifurcation lesion patients. Consistent with our results, a recent study reported that miR30d was upregulated in diabetic cardiomyopathy [15]. Therefore, miR30d may be a promising marker and therapeutic target for various cardiovascular diseases. miR222 has been shown to play an important role in the regulation of vascular inflammation [16]. In this study, we found that circulating level of miR222 was not significantly increased in coronary bifurcation lesion patients compared to nonbifurcation lesion patients. It will be important to further confirm the function of miR222 in coronary bifurcation lesion. Up to now, miR1246 is mainly reported to be involved in cancer development [17, 18]. The role of miR1246 in cardiovascular diseases needs further studies.
5. Conclusions This is the first study using microarray method to investigate the association between serum miRNAs and coronary bifurcation lesion. Evaluation of the screened up- and downregulated miRNAs according to their target mRNAs and biological significance will give some clues for their functional role in coronary bifurcation lesion. Our findings suggest that these
Disease Markers miRNAs may have a role in the pathogenesis of coronary bifurcation lesion and may represent novel biomarkers for the diagnosis and prognosis of coronary bifurcation lesion.
Conflict of Interests The authors declare that they have no conflict of interests.
Authors’ Contribution Yan Liu and Shaoliang Chen designed the study and wrote the paper. Junjie Zhang, Shoujie Shan, Liang Chen, Rong Wang, Jing Kan, and Tian Xu performed the experiments and analyzed the data. All authors read and approved the final paper.
Acknowledgments This study is supported by Jiangsu Provincial Special Program of Medical Science (BL2013001). The authors thank the patients who participated in the study with great enthusiasm, the clinic doctors and nurses, and Wu Jie (Shanghai Kangcheng Biotechnology companies) and Zhang Lei (Shanghai Invitrogen Biotechnology companies) for technical assistance.
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Research Article Analysis of Serum MicroRNAs as Potential Biomarker in Coronary Bifurcation Lesion Yan Liu, Shaoliang Chen, Junjie Zhang, Shoujie Shan, Liang Chen, Rong Wang, Jing Kan, and Tian Xu Department of Cardiology, Nanjing First Hospital, Nanjing Medical University, Changle Road No. 68, Nanjing, Jiangsu 210029, China Correspondence should be addressed to Shaoliang Chen; [email protected] Received 31 October 2014; Revised 11 January 2015; Accepted 17 February 2015 Academic Editor: Varodom Charoensawan Copyright © 2015 Yan Liu et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. Recent evidence suggests that cell-derived circulating miRNAs may serve as the biomarkers of cardiovascular diseases. However, no study has investigated the potential of circulating miRNAs as biomarker for coronary bifurcation lesion. In this study, we aimed to characterize the miRNA profiles that could distinguish coronary bifurcation lesion and identify potential miRNAs as biomarkers of coronary bifurcation lesion. We employed miRNA microarray to screen serum miRNAs profiles of patients with coronary bifurcation lesion and coronary nonbifurcation lesions. We identified 197 miRNAs differentially expressed, including 150 miRNAs upregulated and 47 miRNAs downregulated. We chose 3 miRNAs with significant differences for further testing in 200 patients. RT-PCR analysis of serum samples confirmed that miR30d was upregulated and miR1246 was downregulated in the serum of coronary bifurcation lesion patients compared with nonbifurcation lesion patients. Our findings suggest that these miRNAs may have a role in the pathogenesis of coronary bifurcation lesion and may represent novel biomarkers for the diagnosis and prognosis of coronary bifurcation lesion.
1. Introduction
2. Methods
Coronary artery disease (CAD) is one of the leading causes of death worldwide. The pathogenesis of CAD remains incompletely understood and both genetic and environmental factors are involved in this complex disease [1, 2]. Coronary bifurcation lesion is the most challenging lesion in percutaneous coronary interventional medicine because the rate of restenosis and major adverse cardiac event is significantly higher than nonbifurcation lesion [3]. MicroRNAs (miRNAs) are key regulators of gene expression that have been widely associated with a variety of diseases [4, 5]. Recent evidence suggests that cell-derived circulating miRNAs may serve as the biomarkers of cardiovascular diseases including CAD [6]. However, no study has investigated the potential of circulating miRNAs as biomarker for coronary bifurcation lesion. In this study, we aimed to characterize the miRNA profiles that could distinguish coronary bifurcation lesion and identify potential miRNAs as biomarkers of coronary bifurcation lesion.
2.1. Patients. In the matched case-control study, we recruited 5 patients with coronary bifurcation lesion aged 45–87 years (average 72.4 ± 16.4 years) and 5 control patients with coronary nonbifurcation lesion aged 46–75 years (average 59.6 ± 11.7 years). For large sample validation, we recruited 100 patients with coronary bifurcation lesion aged 45–88 years (average 67.8±10.9 years) and 100 control patients with coronary nonbifurcation lesion aged 40–84 years (average 65.5 ± 10.2 years). Serum samples of all subjects were collected. Coronary bifurcation lesion was defined as a junction of a main vessel and a side branch (with a minimal diameter of 1.5 mm) [7]. Coronary bifurcation lesion patients and control subjects had no other concomitant diseases, including severe cardiomyopathy or valvular heart disease, lung disease, significant cardiac dysfunction or liver and kidney dysfunction, thrombotic disease or blood disease, and connective tissue disease or malignancy or active infection such as hepatitis and tuberculosis.
2 2.2. Serum Samples. The blood was collected from each subject into EDTA anticoagulant tube and centrifuged at 3,000 rpm for 10 min, and the supernatant was stored at −80∘ C. 2.3. RNA Extraction. Total RNA was isolated using TRIzol (Invitrogen) and miRNeasy Mini Kit (QIAGEN) according to the manufacturer’s instructions. RNA was dissolved in nuclease-free water by passing a few times through a pipette tip. RNA quality and quantity were measured by using nanodrop spectrophotometer (ND-1000, Nanodrop Technologies) and RNA integrity was determined by gel electrophoresis. 2.4. RNA Labeling. RNA was labeled using miRCURY Hy3/Hy5 Power Labeling Kit (Exiqon, Vedbaek, Denmark) according to the manufacturer’s guideline. One microgram of each sample was 3 -end-labeled with Hy3TM fluorescent label, using T4 RNA ligase. The mixture was incubated for 30 min at 37∘ C, and the reaction was terminated by incubation for 5 min at 95∘ C. Then, 3.0 𝜇L of labeling buffer, 1.5 𝜇L of fluorescent label (Hy3TM), 2.0 𝜇L of DMSO, and 2.0 𝜇L of labeling enzyme were added into the mixture. The labeling mixture was incubated for 1 h at 16∘ C, and the reaction was terminated by incubation for 15 min at 65∘ C.
Disease Markers Table 1: The characteristics of the patients for microarray analysis.
Age (years) Males Hypertension Diabetes Stroke Current smoker Lesion site LAD Lesion site LM Lesion site RCA Lesion calcification Needing rotablation Restenosis Thrombus TIMI grade 0 TIMI grade 1 Medina classification 111
Coronary bifurcation lesion 𝑛=5
Coronary nonbifurcation lesion 𝑛=5
72.4 ± 16.4 4 (80%) 4 (80%) 0 (0%) 2 (40%) 2 (40%) 4 (80%) 0 (0%) 1 (20%) 0 (0%) 0 (0%) 0 (0%) 1 (20%) 3 (60%) 2 (40%) 0 (0%)
59.6 ± 11.7 2 (40%) 4 (80%) 0 (0%) 2 (40%) 2 (40%) 1 (20%) 4 (80%) 0 (0%) 3 (60%) 1 (20%) 1 (20%) 1 (20%) 2 (40%) 3 (60%) 4 (80%)
2.5. miRNA Microarray. Hy3TM-labeled samples were hybridized on the miRCURYTM LNA Array (v.18.0) (Exiqon) according to the manufacturer’s manual. Following the hybridization, the slides were achieved, washed several times using Wash Buffer Kit (Exiqon), and finally dried by centrifugation for 5 min at 400 rpm. Then, the slides were scanned using the Agilent Microarray Scanner (part number G2505C).
Unsupervised hierarchical clustering and correlation analysis was performed on miRNA data. Data were expressed as mean ± SD and analyzed using SPSS13.0 software. Categorical variables were compared by 𝜒2 test, and continuous variables were compared by 𝑡-test. A value of 𝑃 < 0.05 was considered significant.
2.6. Quantitative RT-PCR. Quantitative PCR was performed on an ABI 7500 system (Applied Biosystems, Foster City, CA). RNA was reverse transcribed with the TaqMan miRNA Reverse Transcription Kit (ABI) according to the manufacturer’s instructions. Subsequently, 2.5 ul of the product was used for detecting miRNA expression by quantitative polymerase chain reaction with TaqMan miRNA Assay Kits (ABI).
3.1. The Characteristics of the Patients. To characterize the miRNAs profiles of coronary bifurcation lesion, we recruited 5 patients with coronary bifurcation lesion and 5 patients with coronary nonbifurcation lesion as the control. The characteristics of these patients were listed in Table 1.
2.7. Data Analysis. The intensity of green signal was calculated after background subtraction and four replicated spots of each probe on the same slide have been averaged. We used Median Normalization Method to obtain “Normalized Data,” Normalized Data = (Foreground − Background)/median; the median was 50 percent quantile of microRNA intensity which was larger than 30 in all samples after background correction. After normalization, the statistical significance of differentially expressed miRNA was analyzed by 𝑡-test. A threshold cut-off value was set to 1 fold change which indicates that the expression of a given miRNA is uniform in both case and control groups. The fold change of greater than 1 indicated upregulated miRNAs, whereas the fold change of less than 1 indicated downregulated miRNAs.
3. Results
3.2. Identification of miRNAs Expression Patterns of Patients with Coronary Bifurcation Lesion. We performed microarray analysis to identify miRNAs expression patterns of patients with coronary bifurcation lesion. We made a heat map to visualize the results of the two-way hierarchical clustering of miRNAs (Figure 1). The color scale shown at the top illustrated the relative expression level of a miRNA: red represented a high relative expression level while green represented a low relative expression level [8]. Furthermore, we made a Volcano plot to illustrate miRNAs differentially expressed between coronary bifurcation lesion and coronary nonbifurcation lesion (Figure 2). We identified 197 miRNAs differentially expressed between coronary bifurcation lesion and coronary nonbifurcation lesion, including 150 miRNAs upregulated and 47 miRNAs downregulated (Supplemental File 1 in Supplementary Material available online at http://dx.doi.org/10.1155/2015/351015).
3 Table 2: Confirmation of differential miRNA expression in 200 patients.
71_exp
1_exp
41_exp
9_exp
42_exp
38_ctl
58_ctl
60_ctl
67_ctl
hsa-miR-4288 hsa-miR-4500 hsa-miR-3184-3p hsa-miR-3664-5p hsa-miR-30d-5p hsa-miR-877-5p hsa-miR-4297 hsa-miR-99b-5p hsa-miR-3920 hsa-miR-222-3p hsa-miR-584-5p hsa-miR-4768-5p hsa-miR-130b-5p hsa-miR-4654 hsa-let-7d-3p hsa-miR-151a-3p hsa-miR-423-3p hsa-miR-155-5p hsa-miR-221-3p hsa-miR-4483 hsa-miR-146b -5p hsa-miR-382-5p hsa-miR-4709-3p hsa-miR-3156-3p hsa-miR-3976 hsa-miR-4456 hsa-miR-5681b hsa-miR-664b-3p hsa-miR-4726-5p hsa-miR-3941 hsa-miR-3686 hsa-miR-4531 hsa-miR-4644 hsa-miR-3611 hsa-miR-1246 hsa-miR-501-3p hsa-miR-937-3p hsa-miR-33b-5p hsa-miR-409-3p ebv-miR-BART17-5p hsa-miR-5582-3p hsa-miR-3605-3p hsa-miR-339-5p hsa-miR-103b hsa-miR-504 hsa-miR-190b hsa-miR-671-3p hsa-miR-652-3p hsa-miR-4667-3p hsa-miR-5195-5p hsa-miR-181d hsa-miR-146a-5p hsa-miR-432-5p hsa-miR-654-3p kshv-miR-K12-3-5p hsa-miR-92b-3p hsa-miR-2115-3p hsa-miR-1266 hsa-miR-3183 hsa-miR-30e-3p hsa-miR-4306 hsa-miR-1255a hsa-miR-3171 hsa-miR-1304-5p sv40-miR-S1-5p hsa-miR-4777-5p kshv-miR-K12-5-5p hsa-miR-5002-5p hsa-miR-630 hsa-miR-1273e hsa-miR-5006-3p hsa-miR-4780 hsa-miR-498 hsa-miR-4725-5p hsa-miR-4472 hsa-miR-4478 hsa-miR-523-5p hsa-miR-522-5p hsa-miR-519c-5p hsa-miR-519b-5p hsa-miR-519a-5p hsa-miR-518e-5p hsa-miR-576-5p hsa-miR-1264 hsa-miR-3680-5p hsa-miR-1285-5p hsa-miR-4784 hsa-miR-204-3p hsv1-miR-H5-3p hsa-miR-520a-5p hsa-miR-4459 hsa-miR-4521 hsa-miR-5007-3p hsa-miR-548an hsa-let-7a-2-3p hsa-miR-5581-3p hsa-miR-3940-5p hsa-miR-574-3p hsa-miR-3938 hsa-miR-4795-5p hsa-miR-4326 hsa-miR-22-5p hsa-miR-4451 hsa-miR-1587 hsa-miR-3146 hsa-miR-4800-5p hsa-miR-3158-5p hsa-miR-4682 hsa-miR-4712-3p hsa-miR-4419b hsa-miR-3935 hsa-miR-4762-5p hsa-miR-1273g-3p hsa-miR-665 hsa-miR-506-5p hsa-miR-1255b-2-3p hsa-miR-548t-3p hsa-miR-548ap-3p hsa-miR-548aa hsa-miR-214-3p hsa-miR-5684 hsa-miR-5197-5p hsa-miR-1972 hsa-miR-761 hsa-miR-125b-2-3p hsa-miR-4694-5p hsa-miR-4503 hsa-miR-3915 hsa-miR-298 hsa-miR-3688-5p hsa-miR-647 hsa-miR-4661-5p hsa-miR-421 hsa-miR-3126-5p hsa-miR-3145-5p hsa-miR-3673 hsa-miR-4254 hsa-miR-5006-5p hsa-miR-767-5p hcmv-miR-UL22A-3p hsa-miR-148b-5p hsa-miR-2115-5p hsa-miR-1272 hsa-miR-4756-5p hsa-miR-4723-5p hsa-miR-3119 hsa-miR-4299 hsa-miR-708-5p hcmv-miR-US25-2-5p hsa-miR-4716-3p hsa-miR-764 hsa-miR-527 hsa-miR-518a-5p hsa-miR-3654 hsa-miR-1255b-5p hsa-miR-3123 hsa-miR-2392 hsa-miR-375 hsa-miR-3160-5p hsa-miR-635 hsa-miR-890 hsa-miR-4445-3p hsa-miR-5698 hsa-miR-4468 hsa-miR-7-2-3p hsa-miR-23c hsa-miR-3911 hsa-miR-620 hsa-miR-192-5p hsa-miR-1204 hsa-miR-3126-3p hsa-miR-20b-3p hsa-miR-3135a hsa-miR-920 hsa-miR-4447 kshv-miR-K12-1-3p hsa-miR-2964a-5p hsa-miR-5002-3p hsa-miR-891a hsa-miR-2681-5p hsa-miR-490-3p hsa-miR-4477a hsa-miR-4275 hsa-miR-500a-5p hsa-miR-622 hsv1-miR-H8-5p hsa-miR-422a hsa-miR-5196-3p hsa-miR-938 hsa-miR-4300 hsa-miR-516b-5p hsa-miR-15a-3p hsa-miR-3926 hsa-miR-516b-3p hsa-miR-516a-3p hsa-miR-424-5p hsa-miR-4305 hsa-miR-3689e hsa-miR-3689b-5p hsa-miR-3689a-5p hsa-miR-4307 hsa-miR-3649 kshv-miR-K12-5-3p hsa-miR-548e hsa-miR-4273 hsa-miR-589-5p hcmv-miR-UL36-5p
Figure 1: Heat map illustrating the expression patterns of upregulated and downregulated miRNAs in patients with bifurcation lesion. Upregulated miRNAs were indicated by red while downregulated miRNAs were indicated by green. The three candidate miRNA markers miR30d, miR222, and miR1246 were underlined in red.
Age (years) Males Smoker Hypertension Diabetes miR30d level miR222 level miR1246 level
Bifurcation lesion (𝑛 = 100)
Nonbifurcation lesion (𝑛 = 100)
𝑃
67.8 ± 10.9 52 52 61 28 0.0258 ± 0.0566 0.1024 ± 0.0616 0.0346 ± 0.0567
65.5 ± 10.2 56 50 60 30 0.0017 ± 0.0006 0.0953 ± 0.0693 0.3004 ± 0.2469
0.377 0.55 0.82 0.76 0.51 0.000 0.881 0.000
Volcano plot (exp. versus ctl.)
6 5
−Log10 (P value)
Color key and histogram 80 40 0 −5 0 5 Value
53_ctl
Count
Disease Markers
4 3 2 1 0 −4
−2
0 2 Log2 fold change
4
Figure 2: miRNAs differentially expressed in patients with bifurcation lesion and patients with nonbifurcation lesion. The volcano plots illustrated miRNAs differentially expressed: dots in black indicted the miRNAs that did not reach significant changes of expression; dots in red on the left indicated the miRNAs that had significant downregulation of expression; and dots in red on the right indicated the miRNAs that had significant upregulation of expression.
3.3. Confirmation of Different miRNAs in Serum of Patients with Coronary Bifurcation Lesion. To confirm our results, we chose three of the most differentially expressed miRNAs, including 2 upregulated (miR30d and miR222) and one downregulated (miR1246), which showed difference by more than 10 times. We enrolled 100 patients with bifurcation lesion and 100 patients with nonbifurcation lesion. As illustrated in Table 2, there were no significant differences in the two groups, including the age, the gender, the status of smoking, hypertension, and diabetes. As shown in Figure 3, RT-PCR analysis showed that circulating serum level of miR30d was profoundly elevated in patients with coronary bifurcation lesion compared to nonbifurcation lesion patients (𝑃 < 0.05). Circulating level of
4
Disease Markers
20000 15000 10000
hsa-miR-4297
hsa-miR-222-3p
hsa-miR-4288
hsa-miR-30d-5p
hsa-miR-423-3p
hsa-miR-2115-3p
hsa-miR-1246
hsa-miR-4644
hsa-miR-3976
0
hsa-miR-3611
5000 hsa-miR-4306
Relative level
25000
Case Control
Figure 3: qRT-PCR analysis of several miRNAs differentially expressed in case and control groups. Case: bifurcation lesion patients; control: nonbifurcation lesion patients. Shown were representative data from three independent experiments.
miR222 was modestly but not significantly increased in coronary bifurcation lesion patients compared to nonbifurcation lesion patients (𝑃 = 0.881). Moreover, serum level of miR1246 was significantly lower in bifurcation lesion patients than in nonbifurcation lesion patients (𝑃 < 0.05). These data confirmed our results of microarray analysis.
4. Discussion Coronary artery disease (CAD) is a multifactorial disease that can be influenced by a multitude of environmental and heritable risk factors. CAD has serious impact on human life and health. Coronary atherosclerosis is a main reason that causes CAD. Atherosclerosis is a chronic and progressive pathologic process characterized by the accumulation of lipid and fibrous elements in the large arteries, which causes a number of cardiovascular-related diseases. The development of atherosclerosis involves the following steps: foam cell formation, fatty streak accumulation, migration and proliferation of vascular smooth muscle cells (VSMCs), and fibrous cap formation. Finally, the rupture of the unstable fibrous cap causes thrombosis that leads to unstable coronary syndromes, myocardial infarction, and stroke. Coronary intervention is an effective means of coronary heart disease treatment. Coronary bifurcation is prone to develop atherosclerotic plaque due to turbulent blood flow and high shear stress. Treatment of coronary bifurcation lesion represents a challenging area in interventional cardiology but recent advances in percutaneous coronary interventions (PCI) have led to the dramatic increase in the number of patients successfully treated percutaneously. Compared with nonbifurcation interventions, bifurcation interventions have a lower rate of procedural success, higher procedural costs, longer hospitalization, and a higher clinical and angiographic restenosis. Introduction of drug-eluting stents (DES) has resulted in a lower event rate and reduction of main vessel
(MV) restenosis. However, side branch (SB) ostial residual stenosis and long-term restenosis remain a problem [9]. MicroRNAs (miRNAs) are a class of short, noncoding, single stranded RNA molecules, approximately 22 nucleotides in length. They negatively regulate gene expression either through inhibition of mRNA translation or by promoting mRNA degradation. Emerging evidence suggests that miRNAs are pivotal regulators of various processes including cell proliferation, differentiation, apoptosis, survival, motility, and morphogenesis [10]. Recently, specific miRNA expression profiles have been reported as a prognostic factor or a predictive factor for disease progression. In particular, serum miRNAs may be used as a biomarker in diagnosis [6]. In pathological process, miRNAs are linked to myocardial hypertrophy, myocardial fibrosis, heart failure, and arrhythmias. A series of miRNAs are involved in pathological progression of coronary heart disease and play pivotal roles in the development of the disease [11–13]. Hoekstra et al. investigated the potential of miRNAs as biomarkers for CAD and reported that unstable angina pectoris patients could be discriminated from stable patients based on the relatively high expression levels of miR-134, miR-198, and miR-370 in peripheral blood mononuclear cells [14]. Therefore, we hypothesized that in CAD serum miRNA levels could be changed and those miRNAs can be used as the biomarkers. In this study, we performed microarray analysis to identify 197 miRNAs differentially expressed in the serum of patients with coronary bifurcation lesion, including 150 miRNAs upregulated and 47 miRNAs downregulated. After a rigorous selection, we screened 3 miRNAs differentially expressed, including downregulated miR1246 and upregulated miR30d and miR222. Further large sample validation in 200 patients demonstrated a distinct serum miRNA expression pattern in patients with coronary bifurcation lesion; miR30d was upregulated and miR1246 was downregulated compared with nonbifurcation lesion patients. Consistent with our results, a recent study reported that miR30d was upregulated in diabetic cardiomyopathy [15]. Therefore, miR30d may be a promising marker and therapeutic target for various cardiovascular diseases. miR222 has been shown to play an important role in the regulation of vascular inflammation [16]. In this study, we found that circulating level of miR222 was not significantly increased in coronary bifurcation lesion patients compared to nonbifurcation lesion patients. It will be important to further confirm the function of miR222 in coronary bifurcation lesion. Up to now, miR1246 is mainly reported to be involved in cancer development [17, 18]. The role of miR1246 in cardiovascular diseases needs further studies.
5. Conclusions This is the first study using microarray method to investigate the association between serum miRNAs and coronary bifurcation lesion. Evaluation of the screened up- and downregulated miRNAs according to their target mRNAs and biological significance will give some clues for their functional role in coronary bifurcation lesion. Our findings suggest that these
Disease Markers miRNAs may have a role in the pathogenesis of coronary bifurcation lesion and may represent novel biomarkers for the diagnosis and prognosis of coronary bifurcation lesion.
Conflict of Interests The authors declare that they have no conflict of interests.
Authors’ Contribution Yan Liu and Shaoliang Chen designed the study and wrote the paper. Junjie Zhang, Shoujie Shan, Liang Chen, Rong Wang, Jing Kan, and Tian Xu performed the experiments and analyzed the data. All authors read and approved the final paper.
Acknowledgments This study is supported by Jiangsu Provincial Special Program of Medical Science (BL2013001). The authors thank the patients who participated in the study with great enthusiasm, the clinic doctors and nurses, and Wu Jie (Shanghai Kangcheng Biotechnology companies) and Zhang Lei (Shanghai Invitrogen Biotechnology companies) for technical assistance.
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