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Ghazi N, Arjmand M, Akbari Z, Owsat Mellati A, Saheb-Kashaf H, Zamani Z. 1H NMR- based metabolomics approaches as non- invasive tools for diagnosis of endometriosis. IJRM 2016; 14 (1) :1-8
URL: http://ijrm.ir/article-1-693-en.html
URL: http://ijrm.ir/article-1-693-en.html
Negar Ghazi1 
, Mohammad Arjmand * 2, Ziba Akbari1 , Ali Owsat Mellati1 , Hamid Saheb-Kashaf3 , Zahra Zamani4
, Mohammad Arjmand * 2, Ziba Akbari1 , Ali Owsat Mellati1 , Hamid Saheb-Kashaf3 , Zahra Zamani4
1- Department of Biochemistry, Zanjan Medical University, Zanjan, Iran
2- Department of Biochemistry, Pasteur Institute of Iran, Tehran, Iran , arjmand1@yahoo.com
3- Navid Medical Center, Tehran, Iran
4- Department of Biochemistry, Pasteur Institute of Iran, Tehran, Iran
2- Department of Biochemistry, Pasteur Institute of Iran, Tehran, Iran , arjmand1@yahoo.com
3- Navid Medical Center, Tehran, Iran
4- Department of Biochemistry, Pasteur Institute of Iran, Tehran, Iran
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Introduction
Endometriosis, is defined by the presence and growth of resembling endometrial tissue outside the uterus (1). Endometriosis affects an estimated 176 million women worldwide usually between the age of 15-49 years, in whom remain undiagnosed and are therefore not treated (2). At present, the gold standard method to diagnose endometriosis is visual inspection by laparoscopy and biopsy of the tissue. However, this is an expensive and invasive procedure.
Diagnosing endometriosis is also a challenge, since only expert gynecologist may diagnose the disease. The extensive efforts made to improve its diagnosis with noninvasive methods that can be justified by in accuracy of clinical examination, and the risks and the diagnostic limitations of laparoscopy. There has been a strong interest in the pathogenesis of endometriosis that is why; new technologies- such as omics science- have emerged to focus on this disease through the use of genomics, proteomics or metabolomics. Metabolomics is a relatively new field of study that focuses on small molecule metabolites (3).
Metabolomics profiling has emerged as a powerful and reliable tool for the identification of total metabolites present in different biological systems under a given physiological condition and changes in metabolite content/ concentration are amplified relative to changes in the transcriptome and proteome (4, 5). The artificial neural network (ANNs), with supervised pattern recognition method, quadratic discriminant analysis (QDA) are sophisticated computational modeling tool that proposed to diagnose the disease with prediction signs in combination with metabolomics data set (6, 7).
In this study, it was hypothesized that metabolic profiles of endometriosis patients are changed compared with healthy group. Proton Nuclear Magnetic Resonance (1H-NMR) Spectroscopy is one of the popular spectroscopic techniques, which can be used to obtain rich signal to identify and quantify complex mixtures of metabolites with little or no sample preparation. Furthermore, only small sample volumes are required, and the test is nondestructive (8).
Materials and methods
Study design and sample source
This prospective cohort study was done in Pasteur Institute, Iran in June 2013. Ethic Committee of the Research Center of Metabolic Disease of Zanjan University of Medical Sciences approved the study protocol. Written informed consent was taken from all participants. 31 randomized infertile women with endometriosis (stage II and III) aged 22-44 years who confirmed by diagnostic laparoscopy in Navid clinical center, Tehran, Iran were enrolled as case group. The control group was consisted of 15 randomized normal women in the same age range. They (control group) had no pelvic pain, pelvic inflammatory disease and base on diagnostic laparoscopy there were no signs of endometriosis.
These women were referred to the infertility center due to male factor infertility. Our exclusion criteria were followed as: receiving any kind of medical or hormonal treatment during the last two months, history of gynecological disorders or surgery. Staging was done according to the American Society for Reproductive Medicine classification of endometriosis (9). Most patients had endometriosis symptoms for six months priors to laparoscopic surgical procedure.
Fasting (more than 8 hr) venous blood samples (5 ml) were collected from all participants in early follicular phase during daytime. Considering the effects of estrogen, it was postulated that the scale of the responses would be greater when measured during the early follicular phase compared to the rest of the menstrual cycle. Blood was allowed to clot and serum was separated by centrifugation at 3,000 rpm for 5 min at 4oC were stored at -80oC until 1H NMR analysis.
1H Nuclear magnetic resonance spectroscopy
Prior to the 1H-NMR experiment, frozen serum samples were thawed at room temperature and vortexted. 540 μL serum was mixed with 60 μL of deuterium oxide (D2O- Pad, kimia Novin Company, Iran) with 3-trimethylsilyl- 1- propanesulfonic acid sodium salt (TMSP- Sigma Company, USA) as internal standard for each sample. 1H-NMR spectra were obtained using Carr- Purcell- Meiboom-Gill (CPMG) protocol in Bruker 400 MHz instrument.
Water peak was suppressed and 128 scan were taken with relaxation time of 3 seconds at 295.5 K temperature for each sample as described earlier (10). Preprocessing of spectra included spectral alignment, baseline correction, elimination of uninformative spectral regions and normalization was done with ProMetab toolbox in MATLAB software (11). The water signal region at 4.7 ppm and regions between 5.4-6.7 ppm, which contained no significant metabolite signal were eliminated (12).
Metabolites and pathway analysis
Expression of different metabolites in endometriosis compared to the controls was analyzed using partial least squares discriminant analysis using MetaboAnalyst 3.0, a web-based analytical pipeline for high-throughput metabolomics studies. The analysis was applied to 46 spectra from 31 endometriosis and 15 control serum samples. The regression coefficient and variable importance in projection score were obtained and then used to identify the metabolites (chemical shifts) contributed most to this classification.
To determine separated metabolites, Human Metabolome Database (HMDB) was used. Chemical shift was feed and corresponding metabolite found out (Figure 1).
Metabolic pathway analysis (Metaboanalyst version 3) was used to assess biochemical pathways that were most affected by endometriosis disease.
Classification model
QDA as a quadratic boundary based classifier and feed forward artificial neural networking (ANNs), which is multilayer classifier were utilized as tools to diagnose the patients with endometriosis and controls. The ANNs model was built using multilayer perceptron with all spectra’s chemical shift between 0-5.5 ppm as inputting data. The model was taught in maximum of 1000 iteration, with twenty neurons in hidden layer and two outputs by Tanagra statistical package.
Performance of the built model was evaluated using 10- fold cross- validation and non- error rate (percent of correctly classified samples) of the validation was reported. For QDA classifier, correct classification rate, positive predictive value, and negative predictive value were estimated to reveal the performance of the classification.
Statistical analysis
Data were analyzed using Student’s t-test by Statistical Package for the Social Sciences, version 16.0, SPSS Inc, Chicago, Illinois, USA (SPSS software).
93-55-8/figure_1.jpg)
Figure 3. Fifteen most important metabolites binned identified by PLS- DA. The colored boxes on the right indicate the relative concentrations of the corresponding metabolite in each group under study. Green color shows decreases and red color shows the increase in concentration of metabolites.
Results
1H- NMR spectroscopy and pattern recognition analysis
Spectra of serum samples showed the variation in spectra between two groups (Figure 2). Most altered metabolic pathways are shown in table I and II. ANN analysis for case group consist training and validation steps. 70% of group observation were selected for training and the remained 30% were verified in the model. The results showed that all 11 samples in training group were recognized as normal and 21 samples in patient group classified as patient, all samples were correctly classified and error rate was zero (Table III). We examined the sensitivity of our model with 30% of remaining samples. Sensitivity discriminate between groups was 50% with error rate of 0.4286 (Table IV).
A 10-fold cross validation was performed (10% of samples left out randomly) to evaluate the performance of QDA classifier. Mean values of classification results for five times replication of 10-fold cross validation are reported in Table V. PLS-DA result shows the good classification between groups with loading plot (Figure 3).
Metabolic pathways relating to these separated metabolites were studied by the help of metabolomics data analyzing (www.metaboanalyst.ca) database.
Table I. Changed metabolites in two groups
93-55-8/table_1.jpg)
Table II. Pathways that were altered in patients with endometriosis compared to controls
93-55-8/table_2.jpg)
Total: the total number of compounds in the pathway; Hits: the actually matched number from
the user uploaded data; Raw p: the original p value calculated from the enrichment analysis; FDR p:
the p value adjusted using False Discovery Rate.
Table III. Multilayer feed forward neural networks classification modeling
93-55-8/table_3.jpg)
Confusion matrix contains training of seventy percent of experimental and control group.
Error rate is frequency of errors, Recall is sensitivity and 1-Precision is specificity rate, which
shows 100 percent sensitivity and specificity.
Error rate= 0.000
Table IV. Multilayer feed forward neural networks Classification prediction test using 30% sample
93-55-8/table_4.jpg)
Error rate is frequency of errors, Recall is sensitivity and 1- Precision is specificity rate. Sensitivity of our control group was 75 percent with 63 percent specificity and 50 percent sensitivity for experimental group with 17 percent specificity.
Error rate= 0.4286
Table V. Quadratic Discriminant Analysis Classification modeling
93-55-8/table_5.jpg)
Mean of quadratic discrimination modeling show 76% correctness. Positive predictive value
is the probability of truly diagnosed patient with endometriosis, i.e. among those who had a
positive screening test, the probability of disease was 71%. Negative predictive value is the
probability of truly diagnosed person with no diseases. The sensitivity of this group test is 78%.
Table VI. Comparison between quadratic discriminant analysis QDA and artificial neural networking ANNs classification
93-55-8/table_6.jpg)
Sensitivity discrimination of two group by QDA is 76%, whereas by ANN is 58%. As seen in table positive and negative predict value is also more sensitive by QDA rather than ANN. QDA: quadratic discriminant analysis ANN: artificial neural networking
93-55-8/figure_2.jpg)
Figure 2. Representative 400 MHz 1H- NMR spectra of serum samples from five controls and five cases. X axis shows the chemical shift of metabolites between 0-5.5 ppm. Y axis shows the intensity of each metabolite peak.
93-55-8/figure_3.jpg)
Figure 2. PLS- DA loading plot (Dots represent the NMR chemical shift of metabolites binnes, Dotes accumulates at center show the similarity of metabolites ppm in two groups, where dotes spotted on distances from centers shows the significant outliers in two group of study).
Discussion
In the present investigation, we applied a 1HNMR- based metabolome profiling approach to investigate metabolic changes in serum from endometriosis patients and model the discriminated metabolites for early diagnose of endometriosis. In this regard, several metabolites including 2-mthoxyestradiol, 2- methoxyestrone, dehydroepiandrostion, androstendione, and cholesterol showed significant increase in the endometriosis group in comparison with the control group.
Meanwhile in juxtaposition, primary bile acids metabolite decreased significantly in the endometriosis group. Generally, there are two ways to synthesize estradiol. The first is to synthesize it from cholesterol and the second is through aromatase enzymes, which convert androgens into the estrogens estradiol (skin and adipose tissue). Various studies have found that in endometriosis, the increase of aromatase enzyme gives rise to increase of the levels of estradiol in adipose tissue and peripheral tissues (13-15). This increase in serum estradiol levels of these patients is not measurable and is usually in the normal range (16).
The increase of the estradiol metabolites, namely 2- methoxyestrone and 2-methoxyestradiol, in serum and urine can be indicative of increase of estradiol in the body. The increase of these metabolites, while the level of estradiol is normal (unpublished data), can be attributed to the increase of estradiol in the peripheral tissues due to aromatase enzyme. Slow and dormant progress of endometriosis is attributed to antiangiogenic properties of 2-methoxyestrone and 2- methoxyestradiol.
This property might be useful in control and treatment of endometriosis (17). In the current study, the levels of these two metabolites were increased. Miller et al found that dehydroepiandrostion (DHEA) metabolites could activate estrogen's alpha and beta receptors thus it leads to increasing estradiol and its metabolites. They found that DHEA and its metabolites are possible contributors in increasing risk of breast cancer in postmenopausal women (18). In the current study, DHEA and androstendione were increased in endometriosis patients.
This increase can be attributed to the stimulant effects of these two metabolites of estradiol. Jana et al recent study have found that oxidative stress is increased in the patients with advanced endometriosis (19). Turgut et al and Melo et al compared advanced stage endometriosis patients with the control group without endometriosis with respect to the oxidative stress markers and found an increase in oxidative stress, which resulted in an increase in total cholesterol in women with advanced stage endometriosis (20, 21). The majority of estrogen is excreted through the liver by primary bile acids and its smaller amount is excreted though the urine (22).
In this study, it was found that reduction in primary bile acids might cause hyperestrogenism as a result of failure of hepatic removal of estrogens from the circulation and consequently increasing growth ectopic endometriosis. In this investigation, the endeavor was to find a new NMR-based metabolome profile marker (outliers) in endometriosis patients through serum metabolites, which are directly or indirectly related to endometriosis disease and model and calibrate the model for early prognosis of the disease. There are many reports concerning the use of ANNs in gynecological diagnosis. Sristatidis et al postulated that ANNs could be used as promising tools in early diagnosis of these types of diseases.
ANNs’s prediction power was also evaluated in in vitro fertilization by the same team (23). Lapeer and colleagues used ANNs for predictive tasks, to find out perinatal parameters influencing birth weight (24). In similar investigation, Atkov et al reported >90% accuracy in diagnosing coronary heart diseases (25). To our knowledge, this is the first report that ANNs and QDA could be used in endometriosis assessments with metabolome profile data.
Conclusion
In conclusion, the models built by QDA and ANNs showed that the two modeling tools can identify serum levels in the patients with endometriosis with 71% and 50% precision, respectively. However, the model designed by QDA methods is more efficient in recognizing endometriosis patients compared to ANNs.
Acknowledgments
We are very grateful to Metabolic Research Center, Zanjan Medical University for financial support of this project.
Conflict of interest
The Authors declares that there is no conflict of interest.
Endometriosis, is defined by the presence and growth of resembling endometrial tissue outside the uterus (1). Endometriosis affects an estimated 176 million women worldwide usually between the age of 15-49 years, in whom remain undiagnosed and are therefore not treated (2). At present, the gold standard method to diagnose endometriosis is visual inspection by laparoscopy and biopsy of the tissue. However, this is an expensive and invasive procedure.
Diagnosing endometriosis is also a challenge, since only expert gynecologist may diagnose the disease. The extensive efforts made to improve its diagnosis with noninvasive methods that can be justified by in accuracy of clinical examination, and the risks and the diagnostic limitations of laparoscopy. There has been a strong interest in the pathogenesis of endometriosis that is why; new technologies- such as omics science- have emerged to focus on this disease through the use of genomics, proteomics or metabolomics. Metabolomics is a relatively new field of study that focuses on small molecule metabolites (3).
Metabolomics profiling has emerged as a powerful and reliable tool for the identification of total metabolites present in different biological systems under a given physiological condition and changes in metabolite content/ concentration are amplified relative to changes in the transcriptome and proteome (4, 5). The artificial neural network (ANNs), with supervised pattern recognition method, quadratic discriminant analysis (QDA) are sophisticated computational modeling tool that proposed to diagnose the disease with prediction signs in combination with metabolomics data set (6, 7).
In this study, it was hypothesized that metabolic profiles of endometriosis patients are changed compared with healthy group. Proton Nuclear Magnetic Resonance (1H-NMR) Spectroscopy is one of the popular spectroscopic techniques, which can be used to obtain rich signal to identify and quantify complex mixtures of metabolites with little or no sample preparation. Furthermore, only small sample volumes are required, and the test is nondestructive (8).
Materials and methods
Study design and sample source
This prospective cohort study was done in Pasteur Institute, Iran in June 2013. Ethic Committee of the Research Center of Metabolic Disease of Zanjan University of Medical Sciences approved the study protocol. Written informed consent was taken from all participants. 31 randomized infertile women with endometriosis (stage II and III) aged 22-44 years who confirmed by diagnostic laparoscopy in Navid clinical center, Tehran, Iran were enrolled as case group. The control group was consisted of 15 randomized normal women in the same age range. They (control group) had no pelvic pain, pelvic inflammatory disease and base on diagnostic laparoscopy there were no signs of endometriosis.
These women were referred to the infertility center due to male factor infertility. Our exclusion criteria were followed as: receiving any kind of medical or hormonal treatment during the last two months, history of gynecological disorders or surgery. Staging was done according to the American Society for Reproductive Medicine classification of endometriosis (9). Most patients had endometriosis symptoms for six months priors to laparoscopic surgical procedure.
Fasting (more than 8 hr) venous blood samples (5 ml) were collected from all participants in early follicular phase during daytime. Considering the effects of estrogen, it was postulated that the scale of the responses would be greater when measured during the early follicular phase compared to the rest of the menstrual cycle. Blood was allowed to clot and serum was separated by centrifugation at 3,000 rpm for 5 min at 4oC were stored at -80oC until 1H NMR analysis.
1H Nuclear magnetic resonance spectroscopy
Prior to the 1H-NMR experiment, frozen serum samples were thawed at room temperature and vortexted. 540 μL serum was mixed with 60 μL of deuterium oxide (D2O- Pad, kimia Novin Company, Iran) with 3-trimethylsilyl- 1- propanesulfonic acid sodium salt (TMSP- Sigma Company, USA) as internal standard for each sample. 1H-NMR spectra were obtained using Carr- Purcell- Meiboom-Gill (CPMG) protocol in Bruker 400 MHz instrument.
Water peak was suppressed and 128 scan were taken with relaxation time of 3 seconds at 295.5 K temperature for each sample as described earlier (10). Preprocessing of spectra included spectral alignment, baseline correction, elimination of uninformative spectral regions and normalization was done with ProMetab toolbox in MATLAB software (11). The water signal region at 4.7 ppm and regions between 5.4-6.7 ppm, which contained no significant metabolite signal were eliminated (12).
Metabolites and pathway analysis
Expression of different metabolites in endometriosis compared to the controls was analyzed using partial least squares discriminant analysis using MetaboAnalyst 3.0, a web-based analytical pipeline for high-throughput metabolomics studies. The analysis was applied to 46 spectra from 31 endometriosis and 15 control serum samples. The regression coefficient and variable importance in projection score were obtained and then used to identify the metabolites (chemical shifts) contributed most to this classification.
To determine separated metabolites, Human Metabolome Database (HMDB) was used. Chemical shift was feed and corresponding metabolite found out (Figure 1).
Metabolic pathway analysis (Metaboanalyst version 3) was used to assess biochemical pathways that were most affected by endometriosis disease.
Classification model
QDA as a quadratic boundary based classifier and feed forward artificial neural networking (ANNs), which is multilayer classifier were utilized as tools to diagnose the patients with endometriosis and controls. The ANNs model was built using multilayer perceptron with all spectra’s chemical shift between 0-5.5 ppm as inputting data. The model was taught in maximum of 1000 iteration, with twenty neurons in hidden layer and two outputs by Tanagra statistical package.
Performance of the built model was evaluated using 10- fold cross- validation and non- error rate (percent of correctly classified samples) of the validation was reported. For QDA classifier, correct classification rate, positive predictive value, and negative predictive value were estimated to reveal the performance of the classification.
Statistical analysis
Data were analyzed using Student’s t-test by Statistical Package for the Social Sciences, version 16.0, SPSS Inc, Chicago, Illinois, USA (SPSS software).
Figure 3. Fifteen most important metabolites binned identified by PLS- DA. The colored boxes on the right indicate the relative concentrations of the corresponding metabolite in each group under study. Green color shows decreases and red color shows the increase in concentration of metabolites.
Results
1H- NMR spectroscopy and pattern recognition analysis
Spectra of serum samples showed the variation in spectra between two groups (Figure 2). Most altered metabolic pathways are shown in table I and II. ANN analysis for case group consist training and validation steps. 70% of group observation were selected for training and the remained 30% were verified in the model. The results showed that all 11 samples in training group were recognized as normal and 21 samples in patient group classified as patient, all samples were correctly classified and error rate was zero (Table III). We examined the sensitivity of our model with 30% of remaining samples. Sensitivity discriminate between groups was 50% with error rate of 0.4286 (Table IV).
A 10-fold cross validation was performed (10% of samples left out randomly) to evaluate the performance of QDA classifier. Mean values of classification results for five times replication of 10-fold cross validation are reported in Table V. PLS-DA result shows the good classification between groups with loading plot (Figure 3).
Metabolic pathways relating to these separated metabolites were studied by the help of metabolomics data analyzing (www.metaboanalyst.ca) database.
Table I. Changed metabolites in two groups
Table II. Pathways that were altered in patients with endometriosis compared to controls
Total: the total number of compounds in the pathway; Hits: the actually matched number from
the user uploaded data; Raw p: the original p value calculated from the enrichment analysis; FDR p:
the p value adjusted using False Discovery Rate.
Table III. Multilayer feed forward neural networks classification modeling
Confusion matrix contains training of seventy percent of experimental and control group.
Error rate is frequency of errors, Recall is sensitivity and 1-Precision is specificity rate, which
shows 100 percent sensitivity and specificity.
Error rate= 0.000
Table IV. Multilayer feed forward neural networks Classification prediction test using 30% sample
Error rate is frequency of errors, Recall is sensitivity and 1- Precision is specificity rate. Sensitivity of our control group was 75 percent with 63 percent specificity and 50 percent sensitivity for experimental group with 17 percent specificity.
Error rate= 0.4286
Table V. Quadratic Discriminant Analysis Classification modeling
Mean of quadratic discrimination modeling show 76% correctness. Positive predictive value
is the probability of truly diagnosed patient with endometriosis, i.e. among those who had a
positive screening test, the probability of disease was 71%. Negative predictive value is the
probability of truly diagnosed person with no diseases. The sensitivity of this group test is 78%.
Table VI. Comparison between quadratic discriminant analysis QDA and artificial neural networking ANNs classification
Sensitivity discrimination of two group by QDA is 76%, whereas by ANN is 58%. As seen in table positive and negative predict value is also more sensitive by QDA rather than ANN. QDA: quadratic discriminant analysis ANN: artificial neural networking
Figure 2. Representative 400 MHz 1H- NMR spectra of serum samples from five controls and five cases. X axis shows the chemical shift of metabolites between 0-5.5 ppm. Y axis shows the intensity of each metabolite peak.
Figure 2. PLS- DA loading plot (Dots represent the NMR chemical shift of metabolites binnes, Dotes accumulates at center show the similarity of metabolites ppm in two groups, where dotes spotted on distances from centers shows the significant outliers in two group of study).
Discussion
In the present investigation, we applied a 1HNMR- based metabolome profiling approach to investigate metabolic changes in serum from endometriosis patients and model the discriminated metabolites for early diagnose of endometriosis. In this regard, several metabolites including 2-mthoxyestradiol, 2- methoxyestrone, dehydroepiandrostion, androstendione, and cholesterol showed significant increase in the endometriosis group in comparison with the control group.
Meanwhile in juxtaposition, primary bile acids metabolite decreased significantly in the endometriosis group. Generally, there are two ways to synthesize estradiol. The first is to synthesize it from cholesterol and the second is through aromatase enzymes, which convert androgens into the estrogens estradiol (skin and adipose tissue). Various studies have found that in endometriosis, the increase of aromatase enzyme gives rise to increase of the levels of estradiol in adipose tissue and peripheral tissues (13-15). This increase in serum estradiol levels of these patients is not measurable and is usually in the normal range (16).
The increase of the estradiol metabolites, namely 2- methoxyestrone and 2-methoxyestradiol, in serum and urine can be indicative of increase of estradiol in the body. The increase of these metabolites, while the level of estradiol is normal (unpublished data), can be attributed to the increase of estradiol in the peripheral tissues due to aromatase enzyme. Slow and dormant progress of endometriosis is attributed to antiangiogenic properties of 2-methoxyestrone and 2- methoxyestradiol.
This property might be useful in control and treatment of endometriosis (17). In the current study, the levels of these two metabolites were increased. Miller et al found that dehydroepiandrostion (DHEA) metabolites could activate estrogen's alpha and beta receptors thus it leads to increasing estradiol and its metabolites. They found that DHEA and its metabolites are possible contributors in increasing risk of breast cancer in postmenopausal women (18). In the current study, DHEA and androstendione were increased in endometriosis patients.
This increase can be attributed to the stimulant effects of these two metabolites of estradiol. Jana et al recent study have found that oxidative stress is increased in the patients with advanced endometriosis (19). Turgut et al and Melo et al compared advanced stage endometriosis patients with the control group without endometriosis with respect to the oxidative stress markers and found an increase in oxidative stress, which resulted in an increase in total cholesterol in women with advanced stage endometriosis (20, 21). The majority of estrogen is excreted through the liver by primary bile acids and its smaller amount is excreted though the urine (22).
In this study, it was found that reduction in primary bile acids might cause hyperestrogenism as a result of failure of hepatic removal of estrogens from the circulation and consequently increasing growth ectopic endometriosis. In this investigation, the endeavor was to find a new NMR-based metabolome profile marker (outliers) in endometriosis patients through serum metabolites, which are directly or indirectly related to endometriosis disease and model and calibrate the model for early prognosis of the disease. There are many reports concerning the use of ANNs in gynecological diagnosis. Sristatidis et al postulated that ANNs could be used as promising tools in early diagnosis of these types of diseases.
ANNs’s prediction power was also evaluated in in vitro fertilization by the same team (23). Lapeer and colleagues used ANNs for predictive tasks
Conclusion
In conclusion, the models built by QDA and ANNs showed that the two modeling tools can identify serum levels in the patients with endometriosis with 71% and 50% precision, respectively. However, the model designed by QDA methods is more efficient in recognizing endometriosis patients compared to ANNs.
Acknowledgments
We are very grateful to Metabolic Research Center, Zanjan Medical University for financial support of this project.
Conflict of interest
The Authors declares that there is no conflict of interest.
Type of Study: Original Article |
References
1. Adamson G, Kennedy S, Hummelshoj L. Creating solutions in endometriosis: global collaboration through the World Endometriosis Research Foundation. J Endometriosis 2010; 2: 3-6.
2. Giudice LC, Kao LC. Endometriosis. Lancet 2004; 364: 1789-1799. [DOI:10.1016/S0140-6736(04)17403-5]
3. Wishart DS, Jewison T, Guo AC, Wilson M, Knox C, Liu Y, et al. HMDB 3.0-The Human Metabolome Database in 2013. Nucleic Acids Res 2013; 41: D801-807. [DOI:10.1093/nar/gks1065]
4. Weljie AM, Newton J, Mercier P, Carlson E, Slupsky CM. Targeted profiling: quantitative analysis of 1H NMR metabolomics data. Anal Chem 2006; 78: 4430-4442. [DOI:10.1021/ac060209g]
5. Kell DB. Metabolomic biomarkers: search, discovery and validation. Expert Rev Mol Diagn 2007; 7: 329-333. [DOI:10.1586/14737159.7.4.329]
6. Amato F, López A, Pe-a-Méndez EM, Vaňhara P, Hampl A, Havel J. Artificial neural networks in medical diagnosis. J Applied Biomed 2013; 11: 47-58. [DOI:10.2478/v10136-012-0031-x]
7. Al-Shayea QK. Artificial neural networks in medical diagnosis. Int J Computer Sci Issues 2011; 8: 150-154.
8. Beckonert O, Keun HC, Ebbels TM, Bundy J, Holmes E, Lindon JC, et al. Metabolic profiling, metabolomic and metabonomic procedures for NMR spectroscopy of urine, plasma, serum and tissue extracts. Nat Protoc 2007; 2: 2692-2703. [DOI:10.1038/nprot.2007.376]
9. "American Society for Reproductive Medicine. Revised American Society for Reproductive Medicine classification of endometriosis: 1996. Fertil Steril 1997; 67: 817-821. [DOI:10.1016/S0015-0282(97)81391-X]
10. Arjmand M, Akbari Z, Taghizadeh N, Shahbazzadeh D, Zamani Z. NMR-based metabonomics survey in rats envenomed by Hemiscorpius lepturus venom. Toxicon 2014; 94C: 16-22.
11. Park Y, Kim SB, Wang B, Blanco RA, Le NA, Wu S, et al. Individual variation in macronutrient regulation measured by proton magnetic resonance spectroscopy of human plasma. Am J Physiol Reg Int Comp Physiol 2009; 297: R202-209. [DOI:10.1152/ajpregu.90757.2008]
12. Nicholson JK, Foxall PJ, Spraul M, Farrant RD, Lindon JC. 750 MHz 1H and 1H-13C NMR spectroscopy of human blood plasma. Anal Chem 1995; 67: 793-811. [DOI:10.1021/ac00101a004]
13. Nothnick WB. The emerging use of aromatase inhibitors for endometriosis treatment. Reprod Biol Endocrinol 2011; 9: 87. [DOI:10.1186/1477-7827-9-87]
14. Ferrero S, Remorgida V, Maganza C, Venturini PL, Salvatore S, Papaleo E, et al. Aromatase and endometriosis: estrogens play a role. Ann N Y Acad Sci 2014; 1317: 17-23. [DOI:10.1111/nyas.12411]
15. Hashim HA. Potential role of aromatase inhibitors in the treatment of endometriosis. Int J womens Health 2014; 6: 671. [DOI:10.2147/IJWH.S34684]
16. Huhtinen K, Desai R, Stahle M, Salminen A, Handelsman DJ, Perheentupa A, et al. Endometrial and endometriotic concentrations of estrone and estradiol are determined by local metabolism rather than circulating levels. J Clin Endocrinol Metab 2012; 97: 4228-4235. [DOI:10.1210/jc.2012-1154]
17. Machado-Linde F, Pelegrin P, Sanchez-Ferrer ML, Leon J, Cascales P, Parrilla JJ. 2-methoxyestradiol in the pathophysiology of endometriosis: focus on angiogenesis and therapeutic potential. Reprod Sci 2012; 19: 1018-1029. [DOI:10.1177/1933719112446080]
18. Miller KK, Al-Rayyan N, Ivanova MM, Mattingly KA, Ripp SL, Klinge CM, et al. DHEA metabolites activate estrogen receptors alpha and beta. Steroids 2013; 78: 15-25. [DOI:10.1016/j.steroids.2012.10.002]
19. Jana SK, Dutta M, Joshi M, Srivastava S, Chakravarty B, Chaudhury K. 1H NMR based targeted metabolite profiling for understanding the complex relationship connecting oxidative stress with endometriosis. BioMed Res Int 2013; 2013: 329058-329167. [DOI:10.1155/2013/329058]
20. Turgut A, Ozler A, Goruk NY, Tunc SY, Evliyaoglu O, Gul T. Copper, ceruloplasmin and oxidative stress in patients with advanced-stage endometriosis. Eur Rev Med Pharmacol Sci 2013; 17: 1472- 1478.
21. Melo AS, Rosa-e-Silva JC, Rosa-e-Silva AC, Poli-Neto OB, Ferriani RA, Vieira CS. Unfavorable lipid profile in women with endometriosis. Fertil Steril 2010; 93: 2433-2436. [DOI:10.1016/j.fertnstert.2009.08.043]
22. Michnovicz JJ, Bradlow HL. Altered estrogen metabolism and excretion in humans following consumption of indole-3-carbinol. Nut Cancer 1991; 16: 59-66. [DOI:10.1080/01635589109514141]
23. Siristatidis CS, Chrelias C, Pouliakis A, Katsimanis E, Kassanos D. Artificial neural networks in gynaecological diseases: Current and potential future applications. Med Sci Monit 2010; 16: RA231-RA236.
24. Lapeer R, Dalton K, Prager R, Forsström J, Selbmann H, Derom R. Application of neural networks to the ranking of perinatal variables influencing birthweight. Scand J Clin Lab Invest 1995; 55: 83-93. [DOI:10.3109/00365519509088454]
25. Atkov OY, Gorokhova SG, Sboev AG, Generozov 8 International Journal of Reproductive BioMedicine Vol. 14. No. 1. pp: 1-8, January 2016.
26. EV, Muraseyeva EV, Moroshkina SY, et al. Coronary heart disease diagnosis by artificial neural networks including genetic polymorphisms and clinical parameters. J Cardiol 2012; 59: 190-194. [DOI:10.1016/j.jjcc.2011.11.005]
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