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Volume 18, Issue 5 (May 2020)
IJRM 2020, 18(5): 347-358 |
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Razi M H, Eftekhar M, Ghasemi N, Sheikhha M H, Dehghani Firoozabadi A. Expression levels of circulatory mir-185-5p, vascular endothelial growth factor, and platelet-derived growth factor target genes in endometriosis. IJRM 2020; 18 (5) :347-358
URL: http://ijrm.ir/article-1-1551-en.html
URL: http://ijrm.ir/article-1-1551-en.html
Mohammad Hossein Razi1 
, Maryam Eftekhar2 , Nasrin Ghasemi3 , Mohammad Hasan Sheikhha * 4, Ali Dehghani Firoozabadi5
, Maryam Eftekhar2 , Nasrin Ghasemi3 , Mohammad Hasan Sheikhha * 4, Ali Dehghani Firoozabadi5
1- Research and Clinical Center for Infertility, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran. Biotechnology Research Center, International Campus, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
2- Research and Clinical Center for Infertility, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran. Abortion Research Center, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
3- Abortion Research Center, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
4- Research and Clinical Center for Infertility, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran. Biotechnology Research Center, International Campus, Shahid Sadoughi University of Medical Sciences, Yazd, Iran. , Sheikhha@yahoo.com
5- Yazd Cardiovascular Research Center, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
2- Research and Clinical Center for Infertility, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran. Abortion Research Center, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
3- Abortion Research Center, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
4- Research and Clinical Center for Infertility, Yazd Reproductive Sciences Institute, Shahid Sadoughi University of Medical Sciences, Yazd, Iran. Biotechnology Research Center, International Campus, Shahid Sadoughi University of Medical Sciences, Yazd, Iran. , Sheikhha@yahoo.com
5- Yazd Cardiovascular Research Center, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
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In addition to VEGF, PDGF has a critical role in angiogenesis and could be essential during vascularization. Although the fundamental molecular mechanisms of PDGF in angiogenesis have not yet been precisely defined, PDGF has attracted much attention from researchers from diverse backgrounds. PDGF and its specific receptors are expressed by natural and tumor cells and have been considered as an anti-angiogenic target for the treatment of solid tumors (9). The PDGF receptor tyrosine kinases, which are known as the α and β subunits, disrupt PDGF-B/β signaling and are associated with significant vascular abnormalities in physiologic and pathologic angiogenesis (10, 11).
Recently, it has been said that microRNAs (miRNAs) are commonly dysregulated in endometriosis. Emerging data show that abnormal miRNA expression in relation to endometriosis may facilitate the development and progression of endometriosis by controlling the proliferation, apoptosis, migration, invasion, and estradiol signal transduction in endometriotic cells (3-5).
Little is known about the pathophysiological significance of miRNA-185 (miR-185) in endometriosis. To investigate the molecular mechanisms by which miR-185 may participate in endometriosis, its target genes were searched. Among them, it was found that there was a highly conserved miR-185 responsive element in the 3ʹ-untranslated region (3ʹ-UTR) of VEGF-A and PDGF. It has been reported that VEGF-A is an important angiogenesis regulator that is highly expressed in tumor tissues such as endometrial tissue, and it is proposed that it is closely associated with aggressive tumor features (12, 13).
We speculate that VEGFA may be the target gene of miR-185. Considering the importance and the role of miRNAs in pathogenesis as well as the diagnosis and progression of various diseases, and the importance of angiogenesis in the progression of endometriosis, the present study evaluated the differential expression of circulating miR-185-5p and predicted the downstream VEGF and PDGF target genes between endometriosis women and healthy controls using real-time quantitative reverse transcription polymerase chain reaction (RT-PCR) to provide evidence of the value of miR-185-5p as a new diagnostic biomarker for endometriosis.
In this study, the expression pattern of miR-185 and its target genes VEGF-A and PDGF were evaluated and compared in whole blood from women with and without endometriosis.
2.8. Ethical consideration
The study proposal was approved by the ethics committee of Shahid Sadoughi university of Medical Sciences, Yazd, Iran (Code: IR.SSU.MEDICINE.REC.1395.300). Written informed consent was obtained from all participants.
2.9. Statistical analysis
Statistical analysis was performed using GraphPad Prism 6 (GraphPad software, San Diego, California, USA). All the experiments were performed at least twice. Using the 2−ΔΔCT method, quantitative RT-PCR data were analyzed. Data were expressed as mean ± SEM and the results were scatter plots with a median value. For statistical comparison between the study groups, the two-tailed nonparametric Mann–Whitney post-hoc and Kruskal–Wallis tests was used. The receiver operating characteristic (ROC) curve was obtained and the area under the curve (AUC) was considered. Correlation analysis was performed using a two-tailed Spearman’s rank correlation. A p-value < 0.05 was considered as statistically significant.
3. Results
Blood samples from 25 women with grade III-IV endometriosis (case group) and 25 women without endometriosis (control group) were screened for the expression of circulating miR-185-5p, VEGF, and PDGF target genes. The demographic characteristics of our study participants are presented in table II. As expected, the two groups had significant differences in the terms of body mass index (BMI) and cancer antigen 125 (p < 0.001). However, the groups did not show significant differences in human epididymis protein 4, carcinoembryonic antigen, white blood cells or hemoglobin (Table II).
For the evaluation of the quality (purity and intactness) and quantity (concentration and extraction efficiency) of extracted total RNA, the NanoDrop ND-1000 and 1.5% agarose gel electrophoresis were used (Figure1 a. The RNA purity was measured using a NanoDrop spectrophotometer, and the A260/A280 and A260/A230 ratios were used as indicators of different contaminants. Ratios between 1.8 and 2.0 for A260/A280 were accepted as indicating pure RNA (Table III). Contamination by DNA and protein was indicated by A260/A280 ratios above 2.0 or below 1.8. For the A260/A230 ratio, the acceptance range was between 1.8 and 2.2 (Table III).
The specificity of the qRT-PCR products of the miR-185, target, and housekeeping genes was confirmed by the existence of a unique peak in the melting curve and the presence of a single band with a predictable size after agarose electrophoresis and SafeView nucleic acid staining (Figure 1 a, b). To evaluate the miRNA expression profiles in whole blood, total miRNAs were isolated, and miRNA expression profiling candidates were examined by Illumina-based deep sequencing. A total of 856 mature miRNAs were distinguished through small non-coding RNA sequencing analysis. The expression profiles of 30 miRNAs were found to be significantly different between the case and control groups (p < 0.016). Of these 30 miRNAs, 15 were upregulated and 15 were downregulated with endometriosis (Figure 2). From these miRNAs, the relative expression of miR-185-5p in the whole blood and plasma of endometriosis women is presented in Figure 3. On the other hand, the expression level of miR-185-5p in plasma was compared between the case and control groups (Figure 3).
3.1. Plasma and whole blood expression levels of miR-185-5p
Comparison of miR-185-5p expression level in plasma and whole blood
The expression levels of miR-185-5p in plasma and whole blood were analyzed using qRT-PCR. The relative expression levels of candidate miRNA are shown in figure 3. Compared with the sera of the control group, the expression of miR-185-5p in the serum was significantly lower in the case group (p < 0.001, RFC = 0.1469); however, no significant change was observed in miR-185-5p expression in whole blood from the cases compared with the control group (p = 0.73, RFC = 1.43). Conversely, plasma and whole blood levels of miR-185-5p were different, and the expression level of miR-185-5p in whole blood was significantly higher than in sera in the case group (p < 0.001) (Figure 3). An ROC curve was generated to analyze the capability of predicting endometriosis in women, and the AUC of miR-185-5p was 0.919 (95% confidence interval (CI): 0.808-1.029, specificity: 0.900, sensitivity: 0.812). The ROC curve analysis of miR-185-5p is shown in Figure 4.
3.2. miR-185-5p as a potential biomarker of endometriosis
To determine the potency of miR-185-5p as a biomarker for endometriosis, an ROC curve was plotted. Remarkably, ROC analysis determined a cut-off value of 0.3750, with high values for sensitivity, specificity, and the AUC of 0.919 for miR-185-5p (P < 0.001; 95% CI: 0.808-1.029), proposing it as a potentially potent predictor for endometriosis (Figure 4).
3.3. Comparison of PDGF and VEGF expression levels in whole blood
The evaluation of the gene targets of PDGF and VEGF in whole blood showed no significant difference in mRNA levels in the case group compared with the controls. The results of RT-PCR demonstrated that compared with the controls, there was no significant decrease or increase in the expression of VEGF and PDGF mRNA in whole blood in the case group compared to the control group (PDGF, p = 0.0976 and VEGF, p = 0.3608). The expression of VEGF-A and PDGF is therefore not able to predict the clinical outcome (Figure 5).
4. Discussion
The present study was undertaken to elucidate the expression level of miR-185-5p in the plasma and whole blood and its angiogenesis-related potential targets (VEGF and PDGF) in the whole blood of 25 women with endometriosis compared with the 25 women without endometriosis. A differential expression analysis of circulating miR-185-5p was conducted and predicted their downstream VEGF and PDGF target genes among the case and control groups using real-time quantitative RT-PCR to provide evidence of the value of miR-185-5p as a new diagnostic biomarker for endometriosis. The goal was to enhance the understanding of the gene expression pattern of miR-185-5p in plasma and whole blood and to assess the potency of this as a biomarker of disease progression in endometriosis.
The results showed that there was a lower expression of miR-185-5p in the plasma of the case group compared to the controls (Figure 3) and that there was no significant difference in the expression of VEGF and PDGF mRNA of whole blood in endometriosis patients compared to the control group (Figure 5). The results show that the mRNA expressions of VEGF and PDGF in whole blood were not statistically significant between the endometriosis and control groups (Figure 5), although increases of 3.12 (PDGF) and 2.33 (VEGF) in relative fold change were observed in the case groups.
To date, few studies have focused on the expression of VEGF and PDGF simultaneously in the whole blood of women suffering from endometriosis. Previous research findings relating to the gene expression pattern of VEGF and PDGF have been inconsistent and contradictory (19-22). The gene expression result of VEGF is similar to the results of Pellicer and colleagues who could not find a significant alternation in the mRNA expression of interleukin-1β and VEGF in women with endometriosis (23). Inconsistent results were identified regarding the gene expression and polymorphisms in the VEGF gene in the progression of endometriosis, which can be ascribed to methodological differences, sample size, qualified control type, using unadjusted risk estimates, and the heterogeneity of the people studied. In some studies, the serum level of the VEGF marker in endometriosis was found to be different from our recent results (24, 25). Some studies have shown an increase in the VEGF expression level and a significant difference in patients with endometriosis compared to the control group (26, 27). In another study, the VEGF level in different phases of the menstrual cycle (in patients who were assumed to have endometriosis) was compared with control groups, and no statistical difference was identified after the calculation of the phase of the cycle (28).
One of the advantages of our data was the simultaneous comparison of VEGF and PDGF expression in whole blood in women with endometriosis compared with the control group. Blood is a tissue and is made up of a variety of cells, each having a different job. In our study, we used whole blood for RNA extraction and miRNA profiling and gene expression quantification of target genes. The buffy coat compose less than 1% of the total volume of the blood, but most of the white blood cells and platelets aggregate in it and therefore it is a good source for RNA extraction. Plasma is considered as an acellular blood component; therefore, nucleic acids extracted from whole blood are mainly extracted from peripheral blood mononuclear cells, including T cells, B cells, NK cells and monocytes (29).
As previously mentioned, PDGF is a platelet-derived growth factor that is an effective mitogen and plays a critical role in the inflammatory response and in the proliferation and differentiation of progenitor cells. It has been confirmed that PDGF plays an essential role in several physiological processes such as wound healing, regeneration, cell proliferation, migration, and angiogenesis. It was reported that PDGF induced the differentiation of embryonic stem cells into endothelial cells (30) and it was indicated that PDGF is also involved in vascular development and tumor angiogenesis in pathological conditions (9, 31). In concert with other proangiogenic factors, PDGF induces the formation and spread of new vessels by recruitment of perivascular cells. It is said that overexpression of PDGF along with VEGF results in pericyte vessel formation and angiogenesis (32). It is also said that combined blockage of VEGF, FGF and PDGF cell signaling pathways suppresses angiogenesis in endometriosis lesions (33).
In our study, despite the expression of PDGF and VEGF being elevated in the whole blood of women with endometriosis, the increased mRNA levels of PDGF and VEGF were not statistically significant. This statistical insignificance could be the result of the small sample size; seemingly insignificant population differences might still find statistical significance. A larger and more varied population would lead to more meaningful results. Based on the above-mentioned reports, it might be anticipated that other miRNAs that target PDGF and VEGF and their receptors could describe molecular and cellular features of endometriotic lesions with a focus on the VEGF- and PDGF-signaling pathways.
According to the previous studies, it appears that angiogenic activity may be increased by the raised level of VEGF in the peritoneal fluid of endometriosis patients. These elevated levels of VEGF and PDGF possibly trigger proangiogenic mediator secretion and neovascularization within the peritoneal environment.
It seems that endometriosis is only related to pelvic inflammation and has nothing to do with the change of VEGF and PDGF levels in circulation. The current knowledge of specific miRNAs that regulate the PDGF and VEGF signal pathways favors the idea that this might be a remunerative target for the development of novel therapeutics. Considering that the subjects in this study had different types of clinical profile that could change the level of VEGF and PDGF in the blood in both the endometriosis and control groups, it can be said that the lack of significant difference observed in VEGF and PDGF could be due to these specific cases. Furthermore, the difference in these controversial results may be due to the small number of people involved in the study.
To avoid any difference in the results, fertile women free of gynecological diseases should be used to form an ideal control group. However, multi-centric studies with a suitable design involving different populations, together with the combined analysis of gene expression in VEGF and PDGF, are necessary to contribute to the understanding of this disease. Nonetheless, the results of the ROC analysis of miR-185-5p expression suggest a potentially non-invasive biomarker in the plasma of endometriosis patients that could reflect disease progression (Figure 4). Therefore, miR-185-5p could potentially serve as a diagnostic biomarker in the prognosis and diagnosis of endometriosis and for evaluation of therapeutic strategies for endometriosis at the molecular level. This will require further and larger-scale studies for confirmation.
5.Conclusion
Our findings proposed miR-185-5p as a novel biomarker and regulator in endometriosis pathogenesis, and these findings support the notion that target therapies against miR-185-5p should have priority in targeting PDGF and VEGF. They are therefore promising tools in therapeutic developments to control the progression and metastasis processes in endometriosis patients. Overall, the results of the statistical analysis suggest miR-185-5p as a potential biomarker of disease activity in endometriosis.
Acknowledgments
This study was financially supported by International Campus of Shahid Sadoughi University of Medical Sciences and Yazd Research and Clinical Center for Infertility.
Conflict of Interest
The authors declare that there are no conflicts of interest.
Full-Text: (436 Views)
- Introduction
In addition to VEGF, PDGF has a critical role in angiogenesis and could be essential during vascularization. Although the fundamental molecular mechanisms of PDGF in angiogenesis have not yet been precisely defined, PDGF has attracted much attention from researchers from diverse backgrounds. PDGF and its specific receptors are expressed by natural and tumor cells and have been considered as an anti-angiogenic target for the treatment of solid tumors (9). The PDGF receptor tyrosine kinases, which are known as the α and β subunits, disrupt PDGF-B/β signaling and are associated with significant vascular abnormalities in physiologic and pathologic angiogenesis (10, 11).
Recently, it has been said that microRNAs (miRNAs) are commonly dysregulated in endometriosis. Emerging data show that abnormal miRNA expression in relation to endometriosis may facilitate the development and progression of endometriosis by controlling the proliferation, apoptosis, migration, invasion, and estradiol signal transduction in endometriotic cells (3-5).
Little is known about the pathophysiological significance of miRNA-185 (miR-185) in endometriosis. To investigate the molecular mechanisms by which miR-185 may participate in endometriosis, its target genes were searched. Among them, it was found that there was a highly conserved miR-185 responsive element in the 3ʹ-untranslated region (3ʹ-UTR) of VEGF-A and PDGF. It has been reported that VEGF-A is an important angiogenesis regulator that is highly expressed in tumor tissues such as endometrial tissue, and it is proposed that it is closely associated with aggressive tumor features (12, 13).
We speculate that VEGFA may be the target gene of miR-185. Considering the importance and the role of miRNAs in pathogenesis as well as the diagnosis and progression of various diseases, and the importance of angiogenesis in the progression of endometriosis, the present study evaluated the differential expression of circulating miR-185-5p and predicted the downstream VEGF and PDGF target genes between endometriosis women and healthy controls using real-time quantitative reverse transcription polymerase chain reaction (RT-PCR) to provide evidence of the value of miR-185-5p as a new diagnostic biomarker for endometriosis.
In this study, the expression pattern of miR-185 and its target genes VEGF-A and PDGF were evaluated and compared in whole blood from women with and without endometriosis.
- Materials and Methods
- 1. Participants
- 2. Blood, plasma, and sample preparation and RNA extraction
- 3. miRNA sequencing
- 4. Reverse transcription and expression analysis
- 5. miRNA sequencing data analysis
- 6. Real-time RT-PCR analysis
- 7. Standard curve and efficiency of PCR
2.8. Ethical consideration
The study proposal was approved by the ethics committee of Shahid Sadoughi university of Medical Sciences, Yazd, Iran (Code: IR.SSU.MEDICINE.REC.1395.300). Written informed consent was obtained from all participants.
2.9. Statistical analysis
Statistical analysis was performed using GraphPad Prism 6 (GraphPad software, San Diego, California, USA). All the experiments were performed at least twice. Using the 2−ΔΔCT method, quantitative RT-PCR data were analyzed. Data were expressed as mean ± SEM and the results were scatter plots with a median value. For statistical comparison between the study groups, the two-tailed nonparametric Mann–Whitney post-hoc and Kruskal–Wallis tests was used. The receiver operating characteristic (ROC) curve was obtained and the area under the curve (AUC) was considered. Correlation analysis was performed using a two-tailed Spearman’s rank correlation. A p-value < 0.05 was considered as statistically significant.
3. Results
Blood samples from 25 women with grade III-IV endometriosis (case group) and 25 women without endometriosis (control group) were screened for the expression of circulating miR-185-5p, VEGF, and PDGF target genes. The demographic characteristics of our study participants are presented in table II. As expected, the two groups had significant differences in the terms of body mass index (BMI) and cancer antigen 125 (p < 0.001). However, the groups did not show significant differences in human epididymis protein 4, carcinoembryonic antigen, white blood cells or hemoglobin (Table II).
For the evaluation of the quality (purity and intactness) and quantity (concentration and extraction efficiency) of extracted total RNA, the NanoDrop ND-1000 and 1.5% agarose gel electrophoresis were used (Figure1 a. The RNA purity was measured using a NanoDrop spectrophotometer, and the A260/A280 and A260/A230 ratios were used as indicators of different contaminants. Ratios between 1.8 and 2.0 for A260/A280 were accepted as indicating pure RNA (Table III). Contamination by DNA and protein was indicated by A260/A280 ratios above 2.0 or below 1.8. For the A260/A230 ratio, the acceptance range was between 1.8 and 2.2 (Table III).
The specificity of the qRT-PCR products of the miR-185, target, and housekeeping genes was confirmed by the existence of a unique peak in the melting curve and the presence of a single band with a predictable size after agarose electrophoresis and SafeView nucleic acid staining (Figure 1 a, b). To evaluate the miRNA expression profiles in whole blood, total miRNAs were isolated, and miRNA expression profiling candidates were examined by Illumina-based deep sequencing. A total of 856 mature miRNAs were distinguished through small non-coding RNA sequencing analysis. The expression profiles of 30 miRNAs were found to be significantly different between the case and control groups (p < 0.016). Of these 30 miRNAs, 15 were upregulated and 15 were downregulated with endometriosis (Figure 2). From these miRNAs, the relative expression of miR-185-5p in the whole blood and plasma of endometriosis women is presented in Figure 3. On the other hand, the expression level of miR-185-5p in plasma was compared between the case and control groups (Figure 3).
3.1. Plasma and whole blood expression levels of miR-185-5p
Comparison of miR-185-5p expression level in plasma and whole blood
The expression levels of miR-185-5p in plasma and whole blood were analyzed using qRT-PCR. The relative expression levels of candidate miRNA are shown in figure 3. Compared with the sera of the control group, the expression of miR-185-5p in the serum was significantly lower in the case group (p < 0.001, RFC = 0.1469); however, no significant change was observed in miR-185-5p expression in whole blood from the cases compared with the control group (p = 0.73, RFC = 1.43). Conversely, plasma and whole blood levels of miR-185-5p were different, and the expression level of miR-185-5p in whole blood was significantly higher than in sera in the case group (p < 0.001) (Figure 3). An ROC curve was generated to analyze the capability of predicting endometriosis in women, and the AUC of miR-185-5p was 0.919 (95% confidence interval (CI): 0.808-1.029, specificity: 0.900, sensitivity: 0.812). The ROC curve analysis of miR-185-5p is shown in Figure 4.
3.2. miR-185-5p as a potential biomarker of endometriosis
To determine the potency of miR-185-5p as a biomarker for endometriosis, an ROC curve was plotted. Remarkably, ROC analysis determined a cut-off value of 0.3750, with high values for sensitivity, specificity, and the AUC of 0.919 for miR-185-5p (P < 0.001; 95% CI: 0.808-1.029), proposing it as a potentially potent predictor for endometriosis (Figure 4).
3.3. Comparison of PDGF and VEGF expression levels in whole blood
The evaluation of the gene targets of PDGF and VEGF in whole blood showed no significant difference in mRNA levels in the case group compared with the controls. The results of RT-PCR demonstrated that compared with the controls, there was no significant decrease or increase in the expression of VEGF and PDGF mRNA in whole blood in the case group compared to the control group (PDGF, p = 0.0976 and VEGF, p = 0.3608). The expression of VEGF-A and PDGF is therefore not able to predict the clinical outcome (Figure 5).
4. Discussion
The present study was undertaken to elucidate the expression level of miR-185-5p in the plasma and whole blood and its angiogenesis-related potential targets (VEGF and PDGF) in the whole blood of 25 women with endometriosis compared with the 25 women without endometriosis. A differential expression analysis of circulating miR-185-5p was conducted and predicted their downstream VEGF and PDGF target genes among the case and control groups using real-time quantitative RT-PCR to provide evidence of the value of miR-185-5p as a new diagnostic biomarker for endometriosis. The goal was to enhance the understanding of the gene expression pattern of miR-185-5p in plasma and whole blood and to assess the potency of this as a biomarker of disease progression in endometriosis.
The results showed that there was a lower expression of miR-185-5p in the plasma of the case group compared to the controls (Figure 3) and that there was no significant difference in the expression of VEGF and PDGF mRNA of whole blood in endometriosis patients compared to the control group (Figure 5). The results show that the mRNA expressions of VEGF and PDGF in whole blood were not statistically significant between the endometriosis and control groups (Figure 5), although increases of 3.12 (PDGF) and 2.33 (VEGF) in relative fold change were observed in the case groups.
To date, few studies have focused on the expression of VEGF and PDGF simultaneously in the whole blood of women suffering from endometriosis. Previous research findings relating to the gene expression pattern of VEGF and PDGF have been inconsistent and contradictory (19-22). The gene expression result of VEGF is similar to the results of Pellicer and colleagues who could not find a significant alternation in the mRNA expression of interleukin-1β and VEGF in women with endometriosis (23). Inconsistent results were identified regarding the gene expression and polymorphisms in the VEGF gene in the progression of endometriosis, which can be ascribed to methodological differences, sample size, qualified control type, using unadjusted risk estimates, and the heterogeneity of the people studied. In some studies, the serum level of the VEGF marker in endometriosis was found to be different from our recent results (24, 25). Some studies have shown an increase in the VEGF expression level and a significant difference in patients with endometriosis compared to the control group (26, 27). In another study, the VEGF level in different phases of the menstrual cycle (in patients who were assumed to have endometriosis) was compared with control groups, and no statistical difference was identified after the calculation of the phase of the cycle (28).
One of the advantages of our data was the simultaneous comparison of VEGF and PDGF expression in whole blood in women with endometriosis compared with the control group. Blood is a tissue and is made up of a variety of cells, each having a different job. In our study, we used whole blood for RNA extraction and miRNA profiling and gene expression quantification of target genes. The buffy coat compose less than 1% of the total volume of the blood, but most of the white blood cells and platelets aggregate in it and therefore it is a good source for RNA extraction. Plasma is considered as an acellular blood component; therefore, nucleic acids extracted from whole blood are mainly extracted from peripheral blood mononuclear cells, including T cells, B cells, NK cells and monocytes (29).
As previously mentioned, PDGF is a platelet-derived growth factor that is an effective mitogen and plays a critical role in the inflammatory response and in the proliferation and differentiation of progenitor cells. It has been confirmed that PDGF plays an essential role in several physiological processes such as wound healing, regeneration, cell proliferation, migration, and angiogenesis. It was reported that PDGF induced the differentiation of embryonic stem cells into endothelial cells (30) and it was indicated that PDGF is also involved in vascular development and tumor angiogenesis in pathological conditions (9, 31). In concert with other proangiogenic factors, PDGF induces the formation and spread of new vessels by recruitment of perivascular cells. It is said that overexpression of PDGF along with VEGF results in pericyte vessel formation and angiogenesis (32). It is also said that combined blockage of VEGF, FGF and PDGF cell signaling pathways suppresses angiogenesis in endometriosis lesions (33).
In our study, despite the expression of PDGF and VEGF being elevated in the whole blood of women with endometriosis, the increased mRNA levels of PDGF and VEGF were not statistically significant. This statistical insignificance could be the result of the small sample size; seemingly insignificant population differences might still find statistical significance. A larger and more varied population would lead to more meaningful results. Based on the above-mentioned reports, it might be anticipated that other miRNAs that target PDGF and VEGF and their receptors could describe molecular and cellular features of endometriotic lesions with a focus on the VEGF- and PDGF-signaling pathways.
According to the previous studies, it appears that angiogenic activity may be increased by the raised level of VEGF in the peritoneal fluid of endometriosis patients. These elevated levels of VEGF and PDGF possibly trigger proangiogenic mediator secretion and neovascularization within the peritoneal environment.
It seems that endometriosis is only related to pelvic inflammation and has nothing to do with the change of VEGF and PDGF levels in circulation. The current knowledge of specific miRNAs that regulate the PDGF and VEGF signal pathways favors the idea that this might be a remunerative target for the development of novel therapeutics. Considering that the subjects in this study had different types of clinical profile that could change the level of VEGF and PDGF in the blood in both the endometriosis and control groups, it can be said that the lack of significant difference observed in VEGF and PDGF could be due to these specific cases. Furthermore, the difference in these controversial results may be due to the small number of people involved in the study.
To avoid any difference in the results, fertile women free of gynecological diseases should be used to form an ideal control group. However, multi-centric studies with a suitable design involving different populations, together with the combined analysis of gene expression in VEGF and PDGF, are necessary to contribute to the understanding of this disease. Nonetheless, the results of the ROC analysis of miR-185-5p expression suggest a potentially non-invasive biomarker in the plasma of endometriosis patients that could reflect disease progression (Figure 4). Therefore, miR-185-5p could potentially serve as a diagnostic biomarker in the prognosis and diagnosis of endometriosis and for evaluation of therapeutic strategies for endometriosis at the molecular level. This will require further and larger-scale studies for confirmation.
5.Conclusion
Our findings proposed miR-185-5p as a novel biomarker and regulator in endometriosis pathogenesis, and these findings support the notion that target therapies against miR-185-5p should have priority in targeting PDGF and VEGF. They are therefore promising tools in therapeutic developments to control the progression and metastasis processes in endometriosis patients. Overall, the results of the statistical analysis suggest miR-185-5p as a potential biomarker of disease activity in endometriosis.
Acknowledgments
This study was financially supported by International Campus of Shahid Sadoughi University of Medical Sciences and Yazd Research and Clinical Center for Infertility.
Conflict of Interest
The authors declare that there are no conflicts of interest.
Type of Study: Original Article |
Subject:
Reproductive Genetics
References
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