Blood metal levels and serum testosterone concentrations in male and female children and adolescents: NHANES 2011–2012
Authors:
Qi Yao aff001; Ge Zhou aff002; Meilin Xu aff003; Jianguo Dai aff001; Ziwei Qian aff001; Zijing Cai aff001; Luyao Zhang aff001; Yong Tan aff002; Rongkui Hu aff002
Authors place of work:
Department of Pathology and Pathophysiology, Nanjing University of Chinese Medicine, Nanjing, Jiangsu Province, China
aff001; Department of Reproductive Medicine, Affiliated Hospital of Nanjing University of Chinese Medicine, Jiangsu Province Hospital of Chinese Medicine, Nanjing, Jiangsu Province, China
aff002; Medical department life science China, GE healthcare China, Beijing, China
aff003
Published in the journal:
PLoS ONE 14(11)
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pone.0224892
Summary
Environmental exposure to metals is ubiquitous, but its relation to androgen hormone levels is not well understood, especially in children and adolescents. This study aimed to explore the relationship between blood metal concentrations (lead, cadmium, total mercury, selenium, and manganese) and serum total testosterone (TT) levels in 6–19-year-old children and adolescents in the National Health and Nutrition Examination Survey (NHANES) 2011–2012. Weighted multivariable linear regression models using NHANES sampling weights were employed to evaluate the association between log-transformed serum TT and each metal categories in male and female children (age 6-11years) and adolescents (age 12–19 years). We established that blood cadmium and manganese levels were associated with significantly higher serum TT levels in the female adolescents. Additionally, the blood selenium levels in male adolescents were related to significantly higher serum TT. No significant associations between blood lead or total mercury levels and TT were observed in children or adolescents of either sex. These findings suggest that environmental exposure to certain metals could affect serum TT levels in adolescents, which might have important implications for the health of adolescents. Further research is required to confirm and extend our present findings.
Keywords:
Blood – Manganese – Metallic lead – cadmium – testosterone – Adolescents – Selenium – Metallic mercury
Introduction
Testosterone is a principal sex hormone needed for the normal physiologic processes during all life stages. In males, testosterone is essential for the development and maintenance of secondary sexual traits [1–2]. Testosterone also influences bone mass, muscle strength, mood, and intellectual capacity [1–2]. In females, testosterone is of crucial importance for bone density and is necessary for normal ovarian and sexual function, libido, energy, and cardiovascular and cognitive functions [3–4].
Testosterone imbalances lead to reproductive dysfunction during multiple life stages in both sexes. Low testosterone levels are related to reduced semen quality in men [5, 6], increased genital malformations [7], and changes in the time of onset and/or progression of puberty [8–9]. On the other hand, high testosterone levels are linked to polycystic ovary syndrome (PCOS) in females [10], increased genital system cancers [11, 12], and altered pubertal development [13, 14]. Therefore, research on the factors affecting testosterone levels in both sexes is needed.
Metals have been shown to interact with testosterone levels. The general population is exposed to low concentrations of metals daily through the consumption of water, foods, supplements, and inhalation of air. Due to widespread metal exposure of humans, a growing concern exists regarding their endocrine-disrupting potential. Non-essential metal elements, such as cadmium, lead, and mercury, have endocrine-disrupting properties even at low concentrations. A positive relationship between environmental cadmium exposure and testosterone levels has also been shown among adult males and females [15–20], and several epidemiologic studies have indicated that environmental lead exposure is associated with increased testosterone levels in U.S., Croatian, and Chinese men [21–23].The research regarding environmental mercury exposure and testosterone levels in humans is limited. A study by Barregârd et al. showed that serum total testosterone (TT) concentrations were positively correlated with cumulative mercury exposure [24]. Essential metals, such as manganese and selenium, can be harmful depending on their concentrations. Rats exposed to low manganese levels had increased testosterone levels, while high manganese levels resulted in decreased testosterone levels [25–27]. Exposing adult male rats to low selenium concentrations resulted in increased testosterone levels, while high levels resulted in decreased testosterone levels [28, 29].
In summary, most studies assessing the reproductive endocrine-disrupting effect of low, environmentally-relevant metal exposures in adults have focused on non-essential metals (cadmium and lead), whereas information on other potential endocrine-disrupting metals is still scant. Moreover, children and adolescents are at the ages where susceptibility to the adverse health effects of endocrine disruptors is most concerning. Few studies have focused on the relationship between environmental metal exposure and endogenous androgen hormone levels in children and adolescents. Therefore, our objective was to examine the potential associations between blood metal (cadmium, lead, mercury, manganese, and selenium) and circulating serum TT levels in a general population sampling of 6–11-year-old children and 12–19-year-old adolescents in the United States.
Materials and methods
Study population
We analyzed the data from the National Health and Nutrition Examination Survey (NHANES) 2011–2012. NHANES is a cross-sectional, U.S.-representative survey conducted annually by the Centers for Disease Control and Prevention (CDC). The goal of NHANES is to assess the health and nutritional status of the general U.S. population. The data were collected by questionnaire surveys, household interviews, physical examinations, and laboratory tests. We analyzed data from a subset of male children (age 6–11 years), male adolescents (age 12–19 years), female children (age 6–11 years), and female adolescents (age 12–19 years). Participants with missing data on blood metal levels, serum TT, and covariates were excluded from the analysis. In the final sample size, we assessed data from 431 male children, 493 male adolescents, 426 female children, and 470 female adolescents. NHANES received approval from the National Center for Health Statistics (NCHS) Ethics Review Board, and informed consent was obtained for all participants.
2.2 Blood sample
Whole venous blood were collected from participants at the Mobile Examination Center (MEC), which were then processed, stored, and shipped to laboratories at the CDC (Atlanta, GA, USA) for analysis. Samples were analyzed for blood metals, serum TT and serum cotinine.
2.3 Serum total testosterone levels
Serum TT levels were analyzed by isotope-dilution liquid chromatography-tandem mass spectrometry. Information regarding the reliability, validation, and quality control of serum TT levels is presented in detail in the NHANES laboratory methods (http://www.cdc.gov/nchs/data/nhanes/nhanes_11_12/TST_G_met.pdf).
2.4 Blood metals
Whole blood lead, cadmium, total mercury, manganese, and selenium concentrations were determined using inductively coupled plasma mass spectrometry-based on quadrupole ICP-MS technology. The methodologic details of blood metal detection and measurements are described in the NHANES laboratory methods(http://www.cdc.gov/nchs/data/nhanes/nhanes_11_12/PbCd_G_met_blood%20metals.pdf). The detection limit for all analytes was constant in the data set. The lower detection limit(LOD) for lead was 0.25 μg/dL, whereas it was 0.16 μg/L for cadmium, 30 μg/L for selenium, 1.06 μg/L for manganese, and 0.16 μg/L for total mercury. Values below the LOD were imputed by LOD and divided by the square root of 2, which provided an imputed value for the individuals who had levels below the LOD.
2.5 Covariates
We examined the following as potential confounding variables: age, race/ethnicity, poverty income ratio (PIR), obesity, seasons of collection, times of venipuncture, and serum cotinine as a biomarker of exposure to environmental tobacco smoke. The selection of these confounders was based on literatures [17, 30].Race/ethnicity was categorized as Non-Hispanic White, Non-Hispanic Black, Hispanic (Mexican American and other Hispanic black), and others. PIR represents the calculated family income to the poverty ratio threshold. Children and adolescents were classified as normal/underweight, overweight, or obese according to their age and sex, in compliance with the criteria defined by NHANES (Body Measures File; https://wwwn.cdc.gov/Nchs/Nhanes/2011-2012/BMX_G.htm). The collection season was obtained from the NHANES demographic data pertaining to the six-month period when the examinations were conducted, which was then classified into two categories, including November 1st–April 30th and May 1st–October 31st. The time of venipuncture, which can be found in the NHANES Fasting Questionnaire File, was categorized as morning, afternoon, or evening sessions. Serum cotinine was measured with isotope dilution-high performance liquid chromatography/atmospheric pressure chemical ionization tandem mass spectrometry (ID HPLC-APCI MS/MS).The methodological details of the detection and measurements of serum cotinine the levels are described in the NHANES laboratory methods (http://www.cdc.gov/nchs/data/nhanes/nhanes_11_12/COT_G_met_cotinine.pdf).
2.6. Statistical analysis
All statistical analyses were performed using Empower (R) (www.empowerstats.com, X&Ysolutions, inc.Boston, MA) and R (http://www.R-project.org) software. Descriptive statistics of participant demographics and concentrations of the metals was calculated. Lead, total mercury, manganese, and selenium were categorized into quartiles because more than 75% of the samples were above LOD. The grouping cut-point for cadmium was determined by the percentage of samples LOD. The low group consisted of all subjects with blood cadmium <LOD, whereas the medium and high groups consisted of equal-sized bins among the detected values. Serum TT was log-transformed for analyses, because the distribution of serum TT was skewed left. Serum cotinine was log-transformed as well. We employed weighted multivariable linear regression models using NHANES sampling weights to evaluate the association between log-transformed serum TT and each metal categories adjusted for the covariates described in section 2.5. Model 1 controlled for age, race and BMI. Model 2 controlled for PIR, seasons of collection, times of venipuncture, and serum cotinine, in addition to the covariates of model 1. Because our dependent variable, serum TT, was log-transformed, the estimated coefficients (β) in the weighted regression models were transformed back by exponentiation of β (exp(β)) and presented as percent differences (equation: % change = [exp(β)-1]× 100). Since the analyses were performed for each subgroup (male children, male adolescents, female children, and female adolescents) separately, the p-values were adjusted for multiple testing using least significant difference (LSD) method. P-values less than 0.05 were considered to be statistically significant.
Results
The characteristics of the study population by age and sex categories are presented in Table 1. The median serum TT levels of male children, male adolescents, female children, and female adolescents were 3.16 ng/dL, 354.67 ng/dL, 4.86 ng/dL, and 23.95 ng/dL, respectively.
As can be seen in Table 2, which shows the distribution of blood metals concentrations by age and sex categories, blood manganese and selenium levels were >LOD for all samples. >75% of the samples had blood lead and total mercury levels >LOD in children and adolescents. 27.8% of the samples had blood cadmium levels >LOD in male children.35.0% of the samples had blood cadmium levels >LOD in female children.51.9% of the samples had blood cadmium levels >LOD in male adolescents.58.7%% of the samples had blood cadmium levels >LOD in female adolescents.
In female adolescents, serum TT was significantly higher for girls in the 4th vs. 1st quartile of lead exposure, but there were no significant trends with increasing quartiles of exposure (adjusted p-trend = 0.14, based on model 1). Blood lead levels did not appear to be associated with serum TT concentrations in male and female children and male adolescents, and consistent trends with increasing quartiles of exposure were not evident (Table 3).
As can be observed in Table 4, serum TT concentrations were positively associated with blood cadmium in female adolescents, and a monotonic increase was seen in the mean serum TT concentration with increasing exposure (adjusted p-trend = 0.004, based on model 1). Significantly higher serum TT levels for the 2nd and 3rd blood cadmium exposure levels (13.24%; 95% CI:3.41%, 24.00%, and 23.15%; 95% CI:6.43%, 42.5%, respectively, based on model 1) compared with the lowest exposure levels were also seen. This pattern of association persisted following an adjustment for age, BMI, race, serum cotinine, time of venipuncture, collection season, family income to poverty ratio, and the p-trend remained significant (adjusted p-trend = 0.002, based on model 2). In male adolescents, serum TT levels were significantly higher in boys in the 3rd vs.1st levels of lead exposure, and the trending p-value was significant (adjusted p-trend = 0.04, based on model1). However, the associations were not significant after adjustment for age, BMI, race, serum cotinine, time of venipuncture, collection season, family income to poverty ratio (adjusted p-trend = 0.62, based on model 2). Blood cadmium did not appear to be associated with serum TT concentrations in male and female children, and consistent trends with increasing exposure were not evident.
In female children, serum TT was significantly higher for girls in the 4thvs.1st quartile of mercury exposure, but there were no signficant trends with increasing quartiles of exposure (adjusted p-trend = 0.10, based on model 1). Blood mercury did not appear to be associated with serum TT in male and female adolescent and male children, and no evidence of consistent trends with increasing quartiles of exposure was established(Table 5).
In male adolescent subjects, the mean serum TT level was higher for boys in the 3rd and 4th quartiles of blood selenium versus those in the 1st quartile, and the trend p-value was significant (adjusted p-trend = 0.0002, based on model 1) (Table 6). However, the quartile-specific increase was significant only for the 4th quartile (43.27%; 95% CI:14.20%, 79.73%, based on model 1). The association were generally consistent with model1 after adjustment for age, BMI, race, serum cotinine, time of venipuncture, season of collection, ratio family income to poverty, and the p-trend remained significant(adjusted p-trend = 0.003 based on model 2). Blood selenium did not appear to be associated with the serum TT level in male and female children and female adolescents, and no evidence of consistent trends with increasing quartiles of exposure was established.
As seen in Table 7, according to model 1, TT was significantly higher in all quartiles of blood manganese than in the lowest quartile in all population subgroups of female adolescents. The trend p-value was significant for female adolescents (adjusted p-trend = 0.001, based on model 1). After adjustment for age, the values of BMI, race, serum cotinine, time of venipuncture, season of collection, ratio of family income to poverty, and the p-trend remained significant (adjusted p-trend = 0.0008, based on model 2). No significant associations were found between serum TT and blood manganese levels in male and female children and male adolescents, and no evidence of consistent trends with increasing quartiles exposure was established.
Discussion
The aim of this study was to investigate the associations between blood metal (lead, cadmium, total mercury, manganese, and selenium) and serum TT levels in male and female children and adolescents. In the present cross-sectional analysis of data from NHANES 2011–2012, blood cadmium and manganese levels were positively associated with serum TT levels in female adolescents. Additionally, blood selenium was positively associated with serum TT levels in male adolescents. No significant associations were observed in the children (male or female).
Circulating testosterone in the body includes sex hormone-binding globulin (SHGB)-bound testosterone, albumin-bound testosterone, corticosteroid-binding globulin (CBG)-bound testosterone, and in an unbound or free form. SHBG-bound testosterone is tightly bound and unavailable to cells. Albumin-bound testosterone and CGB-bound testosterone are weekly bound and dissociate from testosterone rapidly [31]. The term bioavailable testosterone refers to the sum of the albumin-bound, CGB-bound, and free components, which represents the testosterone fraction available to cells. In the present study, we evaluated serum TT, which included both the bioavailable and SHGB-bound forms.
Lead and cadmium, as well-known reproductive toxicants and endocrine disruptor compounds, can cause Leydig cell damage and/or hormone imbalances. In vivo and in vitro studies showed that lead and cadmium might directly affect Leydig cell function by impairing steroidogenesis[32–36].Lead and cadmium also might disrupt hypothalamic-pituitary-testicular axis function, which would alter the hormonal milieu[37–40]. In the present investigation, we were unable to establish an association between blood lead or cadmium levels and serum TT levels among children and adolescent males, which suggested that current exposure levels in our population did not adversely affect testosterone synthesis and regulation.
To our best knowledge, this is the first study to look at the relationships between cadmium exposure and circulating TT levels in adolescent female subjects. The positive association between cadmium and TT levels in female adolescents found in this study was in agreement with the findings reported by Ali I et al. [16] and Nagata C et al. [19]. Ali I et al investigated the relationship between blood cadmium exposure and serum sex hormone levels in 438 postmenopausal Swedish women without hormone replacement therapy, a positive association between blood cadmium and serum TT levels, and an inverse association between blood cadmium and serum estradiol levels and the estradiol/testosterone ratio was found [16]. It is possible that cadmium with LH-induced P450 aromatase activity was responsible for the conversion of testosterone to estradiol. Das and Mukherjee showed that LH-stimulated P450 aromatase activity and P450arom gene expression in carp ovarian follicles were significantly inhibited by cadmium chloride (CdCl2) [41].Unfortunately, gonadotropins and estradiol were not measured in the 2011–2012 NHANES survey. Nagata C et al. found a significantly positive relationship between urinary cadmium and serum TT levels in 164 postmenopausal Japanese women [19]. In a study on rats, exposure to either moderate or high doses of dietary cadmium during gestation led to an increase in serum TT levels in the female rat offspring[42].
We observed a significant positive association between blood manganese and serum TT levels in female adolescents, whereas no association between blood manganese and serum TT levels was found in male adolescents. Several animal studies as reviewed by Dees [43], showed that exposing female and male rat pups to low but increased manganese levels caused the release of hypothalamic luteinizing hormone-releasing hormone (LHRH) in the serum of animals. This effect of manganese on the LHRH-releasing system was consistent with the elevated serum LH, FSH, and gonadal steroid levels in both sexes. Interestingly, sex differences were also observed; males required a higher manganese dose to influence the hypothalamic system compared with females, which indicated that male hypothalamic systems were less sensitive to the influences of manganese. The reason for these sex differences might be due to diversities in the manganese metabolism between the two sexes since male rats can clear the metal over twice faster than females [44].
We also observed a significant positive association between blood selenium and serum TT levels in male adolescents. Selenium is an essential trace element required primarily for the maintenance of spermatogenesis and male fertility [45]. In previous studies, appropriate selenium levels appeared to exert a positive influence on Leydig cells, which thus influenced the secretion of testosterone [46]. An epidemiologic study also revealed that serum TT tended to increase in infertile men supplemented with selenium [47].
Certain limitations of the present study should be acknowledged. First, NHANES is a survey with a cross-sectional design, which restricts the proper interpretation of the causal associations between metal exposures and serum TT levels. Second, no data on free testosterone, SHBG, or other hormones or markers that might have provided clues regarding the mechanisms and/or sites of action of blood metals, were available. Third, the group of 12-to-19-year-old boys and girls classified as adolescents could have included a mixture of pre- and postpubescent children. Lastly, there might have been other confounding factors that we did not evaluate in our analysis.
Conclusions
The results from this study suggest that the blood levels of certain metals were associated with altered serum TT concentrations in male and female adolescents, included in NHANES 2011–2012 data. Our findings pertain to low-level environmental metals exposure and might not be generalizable to environmental or occupational settings where higher metal doses could be encountered. Additionally, altered T levels were found to be linked to a wide range of adverse health effects, but additional epidemiologic human studies, as well as mechanistic studies, are needed to confirm the results of our analysis.
Supporting information
S1 File [xls]
Data name related to this study can be found in S1 File.
S2 File [xls]
Data related to this study can be found in S2 File.
Zdroje
1. Surampudi PN, Wang C, Swerdloff R. Hypogonadism in the aging male diagnosis, potential benefits, and risks of testosterone replacement therapy. Int J Endocrinol. 2012; 2012: 625434. doi: 10.1155/2012/625434 22505891
2. Bassil N, Alkaade S, Morley JE. The benefits and risks of testosterone replacement therapy: a review. Ther Clin Risk Manag. 2009; 5(3): 427–448. doi: 10.2147/tcrm.s3025 19707253
3. Pluchino N, Carmignani A, Cubeddu A, Santoro A, Cela V, Errasti T. Androgen therapy in women: for whom and when. Arch Gynecol Obstet. 2013; 288(4): 731–737. doi: 10.1007/s00404-013-2969-7 23912530
4. Davis SR, Wahlin-Jacobsen S. Testosterone in women—e clinical significance. Lancet Diabetes Endocrinol. 2015; 3(12): 980–992. doi: 10.1016/S2213-8587(15)00284-3 26358173
5. Carlsen E, Giwercman A, Keiding N, Sakkkebaek NE. Evidence for decreasing quality of semen during past 50 years.BMJ. 1992; 305(6854): 609–613. doi: 10.1136/bmj.305.6854.609 1393072
6. Rolland M, Le Moal J, Wagner V, Royère D, thDeMouzon J. Decline in semen concentration and morphology in a sample of 26,609 men close to general population between 1989 and 2005 in France. Hum Reprod. 2013; 28(2): 462–470. doi: 10.1093/humrep/des415 23213178
7. Main KM, Skakkebaek NE, Virtanen HE, Toppari J. Genital anomalies in boys and the environment. Best Pract Res Clin Endocrinol Metab. 2010; 24(2): 279–289. doi: 10.1016/j.beem.2009.10.003 20541152
8. Euling SY, Herman-Giddens ME, Lee PA, Selevan SG, Juul A, Sørensen TI, et al. Examination of US puberty-timing data from 1940 to 1994 for secular trends: panel findings. Pediatrics. 2008; 121 (Suppl 3): S172–191.
9. Zawatski W, Lee MM. Male pubertal development: are endocrine-disrupting compounds shifting the norms? J Endocrinol. 2013; 182(2):R1–R12.
10. Escobar-Morreale HF. Polycystic ovary syndrome: definition, aetiology, diagnosis and treatment. Nat Rev Endocrinol 2018; 14(5): 270–284. doi: 10.1038/nrendo.2018.24 29569621
11. Klap J, Schmid M, Loughlin KR. The relationship between total testosterone levels and prostate cancer: a review of the continuing controversy. J Urol. 2015; 193(2): 403–413. doi: 10.1016/j.juro.2014.07.123 25260832
12. Gann PH, Hennekens CH, Ma J, Longcope C, Stampfer MJ. Prospective study of sex hormone levels and risk of prostate cancer. J Natl Cancer Inst. 1996; 88(16): 1118–1126. doi: 10.1093/jnci/88.16.1118 8757191
13. Cole TJ, Ahmed ML, Preece MA, Hindmarsh P, Dunger DB. The relationship between Insulin-like Growth Factor 1, sex steroids and timing of the pubertal growth spurt. Clin Endocrinol (Oxf). 2015; 82(6): 862–869.
14. Cabrera SM, Rogol AD. Testosterone exposure in childhood: discerning pathology from physiology. Expert Opin Drug Saf. 2013; 12(3): 375–388. doi: 10.1517/14740338.2013.782000 23517636
15. Jurasovic J., Cvitkovic P., Pizent A., Colak B., Telisman S. Semen quality and reproductive endocrine function with regard to blood cadmium in Croatian male subjects. Biometals. 2004; 17, 735–743. 15689116
16. Ali I, Engström A, Vahter M, Skerfving S, Lundh T, Lidfeldt J, et al. Associations between cadmium exposure and circulating levels of sex hormones in postmenopausal women. Environ Res. 2014; 134:265–269. doi: 10.1016/j.envres.2014.08.009 25173093
17. Meeker JD, Rossano MG, Protas B, Padmanahban V, Diamond MP, Puscheck E,et al. Environmental exposure to metals and male reproductive hormones: circulating testosterone is inversely associated with blood molybdenum. FertilSteril. 2010; 93(1): 130–140.
18. Menke A, Guallar E, Shiels MS, Rohrmann S, Basaria S, Rifai N, et al. The association of urinary cadmium with sex steroid hormone concentrations in a general population sample of us adult men. BMC Public Health 2008;8, 72. doi: 10.1186/1471-2458-8-72 18294394
19. Nagata C, Nagao Y, Shibuya C, Kashiki Y, Shimizu H. Urinary cadmium and serum levels of estrogens and androgens in postmenopausal Japanese women.Cancer Epidemiol Biomarkers Prev. 2005; 14(3):705–708. doi: 10.1158/1055-9965.EPI-04-0619 15767353
20. Telisman S., Cvitkovic P., Jurasovic J., Pizent A., Gavella M., Rocic B. Semen quality and reproductive endocrine function in relation to biomarkers of lead, cadmium, zinc, and copper in men. Environ. Health Perspect. 2000; 108(1):45–53. doi: 10.1289/ehp.0010845 10620523
21. Kresovich J. K., Argos M. & Turyk M. E. Associations of lead and cadmium with sex hormones in adult males. Environ. Res. 2015;142: 25–33. doi: 10.1016/j.envres.2015.05.026 26093239
22. Telisman S., Colak B., Pizent A., Jurasovic J. & Cvitkovic P. Reproductive toxicity of low-level lead exposure in men. Environ. Res. 2007;105(2):256–266. doi: 10.1016/j.envres.2007.05.011 17632096
23. Chen C, Wang N, Zhai H, Nie X, Sun H, Han B, et al. Associations of blood lead levels with reproductive hormone levels in men and postmenopausal women: Results from the SPECT-China Study. Sci Rep. 2016; 6: 37809. doi: 10.1038/srep37809 27898110
24. Barregård L, Lindstedt G, Schütz A, Sällsten G. Endocrine function in mercury exposed chloralkali workers. Occup Environ Med. 1994;51(8):536–540. doi: 10.1136/oem.51.8.536 7951778
25. Lee B, Pine M, Johnson L, Rettori V, Hiney JK, Dees WL. Manganese acts centrally to activate reproductive hormone secretion and pubertal development in male rats. ReprodToxicol. 2006;22(4):580–585.
26. Adedara IA, Subair TI, Ego VC, Oyediran O, Farombi EO. Chemoprotective role of quercetin in manganese-induced toxicity along the brain-pituitary-testicular axis in rats. Chem Biol Interact. 2017;263:88–98. doi: 10.1016/j.cbi.2016.12.019 28040552
27. Mohammed AT, Ebraheim LLM, Metwally MMM. Ebselen can Protect Male Reproductive Organs and Male Fertility from Manganese Toxicity: Structural and Bioanalytical Approach in a Rat Model. Biomed Pharmacother. 2018;102:739–748. doi: 10.1016/j.biopha.2018.03.086 29604593
28. Liu L, He Y, Xiao Z, Tao W, Zhu J, Wang B, et al. Effects of Selenium Nanoparticles on Reproductive Performance of Male Sprague-Dawley Rats at Supranutritional and Nonlethal Levels. Biol Trace Elem Res. 2017; 180(1):81–89. doi: 10.1007/s12011-017-0980-8 28261763
29. He Y, Chen S, Liu Z, Cheng C, Li H, Wang M. Toxicity of selenium nanoparticles in male Sprague-Dawley rats at supranutritional and nonlethal levels. Life Sci. 2014; 115(1–2):44–51. doi: 10.1016/j.lfs.2014.08.023 25219884
30. Scinicariello F, Buser MC. Serum Testosterone Concentrations and Urinary Bisphenol A, Benzophenone-3, Triclosan, and Paraben Levels in Male and Female Children and Adolescents: NHANES 2011–2012. Environ Health Perspect. 2016; 124(12):1898–1904. doi: 10.1289/EHP150 27383665
31. de Ronde W, van der Schouw YT, Pols HA, Gooren LJ, Muller M, Grobbee DE, et al. Calculation of bioavailable and free testosterone in men: a comparison of 5 published algorithms. Clin Chem. 2006;52(9):1777–1784. doi: 10.1373/clinchem.2005.063354 16793931
32. P, Pandya C, Bhatt N, Gupta SS. Biochemical and reproductive effects of gestational/lactational exposure to lead and cadmium with respect to testicular steroidogenesis, antioxidant system, endogenous sex steroid and cauda-epididymal functions. Andrologia. 2012; 44(2):92–101. doi: 10.1111/j.1439-0272.2010.01109.x 21933222
33. Thoreux-Manlay A, Le Goascogne C, Segretain D, Jégou B, Pinon-Lataillade G. Lead affects steroidogenesis in rat Leydig cells in vivo and in vitro. Toxicology. 1995; 103(1):53–62. doi: 10.1016/0300-483x(95)03107-q 8525490
34. Cupertino MC, Novaes RD, Santos EC, Neves AC, Silva E, Oliveira JA, et al. Differential Susceptibility of Germ and Leydig Cells to Cadmium-Mediated Toxicity: Impact on Testis Structure, Adiponectin Levels, and Steroidogenesis. Oxid Med Cell Longev. 2017;2017:3405089. doi: 10.1155/2017/3405089 29422988
35. Laskey JW, Phelps PV. Effect of cadmium and other metal cations on in vitro Leydig cell testosterone production. Toxicol Appl Pharmacol. 1991; 108(2):296–306. doi: 10.1016/0041-008x(91)90119-y 1850171
36. Zhang Q, Zou P, Zhan H, Zhang M, Zhang L, Ge RS, Huang Y. Dihydrolipoamide dehydrogenase and cAMP are associated with cadmium-mediated Leydig cell damage. Toxicol Lett. 2011; 205(2):183–189. doi: 10.1016/j.toxlet.2011.06.003 21699967
37. Lafuente A, Márquez N, Pérez-Lorenzo M, Pazo D, Esquifino AI. Pubertal and postpubertal cadmium exposure differentially affects the hypothalamic-pituitary-testicular axis function in the rat. Food Chem Toxicol. 2000; 38(10):913–923. doi: 10.1016/s0278-6915(00)00077-6 11039325
38. Ronis MJ, Badger TM, Shema SJ, Roberson PK, Shaikh F. Reproductive toxicity and growth effects in rats exposed to lead at different periods during development. Toxicol Appl Pharmacol. 1996;136(2):361–371. doi: 10.1006/taap.1996.0044 8619245
39. Lafuente A, Márquez N, Pérez-Lorenzo M, Pazo D, Esquifino AI. Cadmium effects on hypothalamic-pituitary-testicular axis in male rats. Exp Biol Med (Maywood). 2001; 226(6):605–611.
40. Gandhi J, Hernandez RJ, Chen A, Smith NL, Sheynkin YR, Joshi G, et al. Impaired hypothalamic-pituitary-testicular axis activity, spermatogenesis, and sperm function promote infertility in males with lead poisoning. Zygote. 2017; 25(2):103–110. doi: 10.1017/S0967199417000028 28185602
41. Das S, Mukherjee D. Effect of cadmium chloride on secretion of 17β-estradiol by the ovarian follicles of common carp, Cyprinus carpio. Gen Comp Endocrinol. 2013; 181: 107–114. doi: 10.1016/j.ygcen.2012.10.010 23146792
42. Davis J, Khan G, Martin MB, Hilakivi-Clarke L. Effects of maternal dietary exposure to cadmium during pregnancy on mammary cancer risk among female offspring.J Carcinog. 2013; 12:11. doi: 10.4103/1477-3163.114219 23858299
43. Dees WL, Hiney JK, Srivastava VK. Influences of manganese on pubertal development. J Endocrinol. 2017; 235(1): R33–R42. doi: 10.1530/JOE-17-0237 28720645
44. Zheng W, Kim H, Zhao Q. Comparative toxicokinetics of manganese chloride and methylcyclopentadienyl manganese tricarbonyl (MMT) in Sprague-Dawley rats. Toxicol Sci. 2000; 54(2): 295–301. doi: 10.1093/toxsci/54.2.295 10774811
45. Ursini F, Heim S, Kiess M, Maiorino M, Roveri A, Wissing J, et al. Dual function of the selenoproteinPHGPx during sperm maturation. Science. 1999; 285(5432): 1393–1396. doi: 10.1126/science.285.5432.1393 10464096
46. Shi L, Song R, Yao X, Ren Y. Effects of selenium on the proliferation, apoptosis and testosterone production of sheep Leydig cells in vitro. Theriogenology. 2017; 93: 24–32. doi: 10.1016/j.theriogenology.2017.01.022 28257863
47. Safarinejad MR, Safarinejad S. Efficacy of selenium and/or N-acetyl-cysteine for improving semen parameters in infertile men: a double-blind, placebo controlled, randomized study. J Urol. 2009; 181(2): 741–751. doi: 10.1016/j.juro.2008.10.015 19091331
Článok vyšiel v časopise
PLOS One
2019 Číslo 11
- Metamizol jako analgetikum první volby: kdy, pro koho, jak a proč?
- Nejasný stín na plicích – kazuistika
- Masturbační chování žen v ČR − dotazníková studie
- Úspěšná resuscitativní thorakotomie v přednemocniční neodkladné péči
- Kombinace metamizol/paracetamol v léčbě pooperační bolesti u zákroků v rámci jednodenní chirurgie
Najčítanejšie v tomto čísle
- A daily diary study on maladaptive daydreaming, mind wandering, and sleep disturbances: Examining within-person and between-persons relations
- A 3’ UTR SNP rs885863, a cis-eQTL for the circadian gene VIPR2 and lincRNA 689, is associated with opioid addiction
- A substitution mutation in a conserved domain of mammalian acetate-dependent acetyl CoA synthetase 2 results in destabilized protein and impaired HIF-2 signaling
- Molecular validation of clinical Pantoea isolates identified by MALDI-TOF