Follow-Up Study of 17-β Estradiol, Prolactin and Progesterone with the Kinetics and Prevalence of T. gondii Infection in Pregnant Women
by
, ,
Yithzel Guadalupe Luna Rojas
1
,
Eva Elizabet Camarena Pulido
1,
Laura Rocío Rodríguez-Pérez
2 and
María de la Luz Galván-Ramírez
2,* 1
Departamento de Ginecología y Obstetricia, Hospital Civil Juan I. Menchaca, Guadalajara 44340, Mexico
2
Departamento de Microbiología y Patología, Centro Universitario de Ciencias de la Salud, Universidad de Guadalajara, Guadalajara 44340, Mexico
*
Author to whom correspondence should be addressed.
Curr. Issues Mol. Biol. 2024, 46(6), 5701-5711; https://doi.org/10.3390/cimb46060341
Submission received: 4 May 2024
/
Revised: 1 June 2024
/
Accepted: 2 June 2024
/
Published: 7 June 2024
(This article belongs to the Special Issue Molecular Research in Reproductive Biology, 2nd Edition)
Abstract
:Toxoplasmosis is an infection caused by the parasite Toxoplasma gondii. One-third of the world’s population has come into contact with this parasite. In Mexico, the prevalence is between 15% and 50% in the general population and 34.9% in women with high-risk pregnancies. In pregnancy, the highest incidence of infection occurs in the third trimester and fetal damage is inversely proportional to gestational age. Maternal hormones play a fundamental role in the immune response. There are very few studies, with controversial results, on the levels of increased hormones and their relationship to the kinetics of T. gondii infections during pregnancy. The aim was to determine the serum levels of 17-β estradiol, prolactin, and progesterone, and their association with anti-T. gondii antibodies’ kinetics in pregnancy. Fifty-two pregnant patients were studied. A questionnaire with sociodemographic and clinical aspects was used. Afterward, 10 mL of venous blood was collected by venipuncture every trimester. The concentrations of 17-β estradiol, progesterone, and prolactin were measured, using the ELISA method. In addition, anti-Toxoplasma IgG and IgM antibodies were also determined in the first, second, and third trimester. The prevalence of anti-Toxoplasma IgG antibodies was 26.92% in the first and second trimester and 32.7% in the third trimester. In seropositive women, 17-β estradiol increased in the second and third trimesters of pregnancy. Progesterone increased significantly p < 0.039 in the third trimester in these women, while prolactin increased in the second trimester with a statistical significance of p < 0.021. In addition, 17-β estradiol, progesterone, and prolactin are associated with T. gondii infection during pregnancy. New studies are necessary to clarify the specific mechanisms of immune response related to these hormones during pregnancy.
1. Introduction
Toxoplasmosis is a disease caused by the protozoan Toxoplasma gondii (T. gondii). The worldwide prevalence depends on geographic location, dietary habits, and cohabitation with cats [1]. The infection can be asymptomatic. The worldwide prevalence in women varies between 7% and 51%. In women who have had at least one abortion, the prevalence is 17–52.3% [2]. In Mexico, a meta-analysis was carried out in 2012 in which the average prevalence was 27.97% and the weighted prevalence was 19.27%. The latter was higher in women with a history of miscarriage (35.13%), immunocompromised patients (28.54%), and psychiatric patients (38.52%) [3].
Congenital toxoplasmosis occurs when a woman acquires the infection for the first time in a period shortly before or during pregnancy [1,2,3]. In the acute phase, the tachyzoites of T. gondii penetrate the placental barrier and infect the fetus. Nonetheless, maternal immunity exists if contact with the parasite has already taken place before pregnancy.
The incidence of primary infection in pregnancy varies between 1 in 310 to 1 and 10,000 pregnancies. The probability of transplacental infection and the clinical manifestations depend on the trimester of pregnancy in which the mother becomes infected, and the severity of damage to the fetus is inversely proportional to the gestational age at which the infection occurs [4,5,6,7,8,9,10].
Regarding 17-β estradiol (E2), pregnancy is considered as a state of immunological tolerance. Several mechanisms have been found to contribute to this tolerance [11,12]. There is evidence of progressive maternal immunoregulation at the interface, which affects the decidua and placentation. Some specific gestational factors, such as maternal hormones, can modulate the maternal immune response and influence the activation of macrophages and lymphocytes in the decidua [13]. There is a marked increase in E2 and progesterone (P4) in the second and third trimesters of pregnancy, and it is during this period that the prevalence of Toxoplasma infection is the highest [14]. Endocrine changes during pregnancy, as well as the size and development of the placenta, affect the mother’s ability to fight infections [15]. E2 is mainly synthesized in the ovaries, breast tissue, endometrium, and brain. E2 plays an important role in the menstrual cycle and human reproduction. On the other hand, increased levels of E2 have also been associated with toxoplasmosis during pregnancy [16,17,18,19].
Progesterone (P4) is synthesized in the ovaries and the corpus luteum. It is mainly involved in the second phase of the menstrual cycle and is vital in the first weeks of pregnancy [20]. Progesterone plays an important role in regulating the immune cells, which are essential for pregnancy maintenance. The development of the decidua also depends on progesterone, being crucial for the trophoblast implantation [21,22]. A decrease in serum P4 levels has been observed in pregnant women infected with T. gondii; however, the mechanism by which this modulation occurs is still unknown [22,23,24].
Prolactin (Prl) is secreted by the pituitary gland, but it is also produced by the placenta, B and T lymphocytes, and NK cells. Its secretion is controlled by the PrL Inhibiting Hormone (PIH), which is dopamine. Both men and women have low serum levels of this hormone [23,24]. Hyperprolactinemia is a situation in which high levels of Prl are present in the blood, which is very common in women, especially during pregnancy [25,26]. The differences observed in the prevalence of some parasitic infections between men and women may indicate the possible role of sex hormones in the immunity against these parasites. One of the hormones that exhibit a broad spectrum of biological activities, including immunomodulatory effects, is Prl [25,26,27]. In addition, it has been documented, # that female patients with hyperprolactinemia have a lower prevalence rate of T. gondii infections compared to those with hipoprolactinemia [27].
The aim was to determine the serum levels of 17-β estradiol, prolactin, and progesterone, and their association with anti-T. gondii antibodies kinetics in pregnancy.
2. Materials and Methods
2.1. Study Design
It was an observational and longitudinal clinical study in pregnant women. The target population were patients attending prenatal obstetric appointments at the Nuevo Hospital Civil de Guadalajara “Dr. Juan I. Menchaca” from 2021 to 2023. The patients were invited to participate and were informed about the study. Patients who agreed signed an informed consent form.
2.2. Inclusion Criteria
A total of sixty pregnant women, with a range of age of 17 to 42 years, participated in this study. The women were informed about all aspects of the study. Those who agreed to participate signed their informed consent. A questionnaire was then completed, which included answers on the risk factors for T. gondii infection. In addition, 10 mL of venous blood were collected at weeks 5–13.6 (first trimester), 14–25.6 (second trimester), and 26–40 (third trimester) of pregnancy.
2.3. Exclusion Criteria
Women who decided not to participate were excluded. In addition, women with an obstetric emergency, e.g., severe pre-eclampsia, eclampsia, placental abruption, uterine rupture, inevitable pregnancy loss, ectopic pregnancy, and multiple pregnancies were also excluded.
2.4. Elimination Criteria
Eight patients that stopped showing up to the follow-up appointments and did not show up for the next blood draw were excluded.
2.5. Questionnaire
Occupation (household, professional, employee, student, and merchant). Education (none, elementary school, middle school, high school, bachelor’s degree, master’s degree). Living situation (rural or urban). Features of the house (dirt floor, mosaic floor, electricity, water, and drainage). Contact with cats in the house (no, yes, indoors or outdoors, use of a litter box). Handling cat feces (with gloves, without gloves). Handling food (washed or unwashed vegetables and fruit, raw or cooked vegetables). Background information (blood transfusions, miscarriage or stillborn) Clinical features (visual disturbances, headaches, and lymphadenopathy).
2.6. Diagnostic Laboratorio
Blood Samples: The blood that was drawn was centrifuged to obtain the serum and stored at a temperature of −20 °C until processed.
2.6.1. Immunoenzyme Assay (ELISA) for Anti-Toxoplasma IgG and IgM
ELISA kits were used (Platelia TM Toxo; Bio-Rad, IgG catalog # 72840 and IgM 72841, Marnes-la-Coquette, France). The standard control and samples were diluted 1/21. The microplate is sensitized with the inactivated T. gondii antigen. IgG and IgM antibodies against Toxoplasma were determined in the first, second, and third trimester of pregnancy. The antibody concentrations were determined according to the manufacturer’s instructions. The coefficient of variation intra-assay and inter-assay for IgG was 5.96% and 10.2% respectively, the sensitivity of IgG was 98.3%, and the specificity was 100%. Titer ≥ 9 IU/mL was considered positive. Regarding the IgM antibodies, only 1/60 samples (1.96%) were positive. Concerning IgM, the intra-assay and the inter-assay coefficient of variation were 5.96% and 10.1% respectively. The sensitivity was 93% and the specificity was 99.9%.
2.6.2. Immunoenzyme Assay (ELISA) for Serum Levels of 17β-Estradiol, Prolactin and Progesterone
The serum levels of E2, Prl, and P4 were determined by a Monoclonal immunoenzyme assay (ELISA Monobind, Inc, Lake Forest, CA, USA, E2 4925-300, PRL 725-300, and PG 4825-300). All samples were analyzed in duplicate. The three assay tests had the same principle. Samples, standards, and controls were duplicated and analyzed according to the manufacturer’s instructions. The samples analyzed were from the first, second, and third trimesters of pregnancy. 17β-estradiol had a sensitivity of 95% and a specificity of 98%. The inter-assay coefficient of variation was 8.6%. For progesterone, the sensitivity was 95% and the specificity 96%. The Inter-assay coefficient of variation was 6.2%. And for Prl the sensitivity was 95% and the specificity 96%. The inter-assay coefficient of variation was 5.2%. Titer ≥ 1.00 were considered positive.
2.7. Statistical Analysis
Data analysis was performed using SPSS software version 27 (IBM, Los Angeles, CA, USA). Variables such as IgG anti-Toxoplasma antibodies between positive and negative pregnant women were analyzed using Pearson’s chi-square test or Fisher’s exact probability using an ANOVA test. The risk of infection due to Toxoplasma exposure was determined using odds ratio tests with a 95% confidence interval to assess the risk, and the significance level was p < 0.05.
3. Results
3.1. Risk Factors and Sociodemographic Features
A questionnaire with sociodemographic data, risk factors, and comorbidities was answered by 52 patients, who attended prenatal appointments in the first, second, and third trimesters. Therefore, the results of anti-Toxoplasma IgG, E2, P4, and Prl concentrations were obtained per trimester.
The association of anti-Toxoplasma antibodies was examined with occupation (household, professional, employee, student, and merchant); education (none, elementary school, middle school, high school, bachelor’s degree, master’s degree); living situation (rural or urban); features of the house (dirt floor, mosaic floor, electricity, water, and drainage); contact with cats in the house (no, yes, indoors or outdoors, use of a litter box); handling cat feces (with gloves, without gloves); and handling food (washed or unwashed vegetables and fruit, raw or cooked vegetables). No statistically significant difference was found in the socio-demographic data between seropositive and seronegative patients. See Supplementary Table S1.
Clinical Features
The mean age was 24.9 ± 5.61 years, with a range of 17 to 35 years, and 15/52 (28.84%) of patients had a prior history of miscarriage or stillborn, of which 33.3% were positive for anti-T. gondii IgG. The risk of having a miscarriage or stillborn was 1.8 times higher in patients seropositive to IgG (OR: 1.16, CI 95%: 0.28–4.48). Background information included clinical features (visual disturbances, headaches, and lymphadenopathy, miscarriage or stillborn). No significant risk was found related to seropositivity and visual disturbances, headaches, or lymphadenopathy.
3.2. Prevalence of Anti-Toxoplasma Antibodies
By pregnancy trimester, seropositivity for anti-Toxoplasma IgG was 14/52 (26.92%) in the first and second trimesters and 17/52 (32.7%) in the third trimester. Concerning IgM, only 1/52 (1.92%) were positive in the first trimester. High levels of anti-Toxoplasma antibodies were observed in the first trimester. The majority increased more than four times compared to the cut-off value, and a decrease during the second and third trimesters was observed in Figure 1.
The comparison of the serum levels of E2, Prl, and P4 in patients seropositive to anti-Toxoplasma IgG antibodies, against those that were seronegative, was performed in each trimester of pregnancy and showed the following significant result: an important rise in Prl levels in the second trimester with a p value < 0.021, and increase in P4 levels in the third trimester with a p value < 0.039. The colored lines correspond to each of the seropositive patients.
3.3. Hormonal Levels
The concentration of IgG and IgM antibodies was reported in IU/mL according to the manufacturer’s instructions. Similarly, E2 concentration values were expressed in pg/mL, while those of Prl and P4 were expressed in ng/mL. The analysis of the ranges and mean standard deviation of the anti-Toxoplasma antibodies and hormones can be found in Table 1.
To determine the hormonal behavior of E2, Prl, and P4, related to the positivity of anti-T. gondii IgG antibodies, by trimester of pregnancy, an ANOVA test was calculated (Figure 2).
In the second trimester, Prl showed a significant increase (p < 0.02), while P4 was also raised, but without reaching statistical significance, with a p value of 0.053. On the other hand, P4 showed a significant increase (p < 0.039) in the third trimester of pregnancy (Table 2, Table 3 and Table 4). The concentration of E2, P4, and Prl and association with positivity of anti-Toxoplasma antibodies are shown in Figure 2 and Figure 3 and Table 2, Table 3 and Table 4.
E2 levels in all patients show a gradual increase of this hormone per trimester, being slightly more pronounced in the third trimester. In addition, P4 levels increased significantly in the second and third trimesters, while Prl increased similarly, only more pronounced, in the second trimester (Figure 4).
4. Discussion
The prevalence of T. gondii infection in the population studied was 26.9% in the first and second trimesters, rising to 32.7% in the third trimester. This was lower than the 34.9% found in women with high-risk pregnancies in 1995 and close to the 26.01% found in the control group of the same population. On the other hand, only one case of IgM seropositivity was found (1.92%); lower than the 20.7% found in 350 women with high-risk pregnancies and close to the 1.9% in the control group of this study [8]. This could be due to the increased awareness, over the last 30 years, of the risks of neonatal infection during pregnancy. However, the incidence found is higher than that reported in another study from Venezuela, where IgM was positive in 0.26–0.47% of the studied population [2].
Regarding hormonal E2 levels, a trend towards higher E2 levels was observed in women seropositive to IgG, without reaching statistical significance. This finding is similar to that of pregnant women from Iraq and Egypt, where higher E2 levels were associated with chronic T. gondii infection [20,22]. This suggests that E2 increases maternal susceptibility to T. gondii infections [19].
As for acute infection, only one case was IgM-positive, so we could not compare our results between IgG seropositive and acute infections and could not predict whether E2 levels were related to the kinetics of the acute illness. In studies conducted in vitro, pretreatment with E2 on THP-1 cells infected with T. gondii increased parasite replication [16,17]. In addition, another study found that E2 can promote the infection by T. gondii in vitro and in vivo, which is related to the Toxoplasma gene Tg-HSD [18]. On the other hand, E2 can decrease the inflammation [28,29,30].
The P4 levels were higher in the seropositive IgG patients, compared to the seronegative patients, in the second and third trimesters of pregnancy. These findings are similar to those reported in Iraq in pregnant women infected with T. gondii, where an increase in P4 levels was found in the second and third trimesters compared to controls [21]. Furthermore, low P4 levels in pregnant patients with toxoplasmosis are associated with adverse effects caused by the infection, as was demonstrated [13]. On the other hand, it has been suggested that the T. gondii membrane receptor protein (TgPGRMC), located in the parasite’s mitochondria, may be affected by P4, inhibiting its replication [24].
These results are consistent with those found in a study executed in vivo, in which P4 levels were strongly associated with chronic infection [21]. In another study carried out on in vitro astrocytes that were pretreated with P4 and infected by T. gondii, it was found that the P4 treatment reduced the parasitic replication significantly, compared to the control group [15].
As for the results of Prl levels, they increased in the second and third trimesters of pregnancy in the overall population. However, Prl levels were significantly higher in IgG-positive women in the second trimester, while an important decrease is observed, in this group, in the third trimester. Similar results were reported in a study carried out on pregnant women with T. gondii infection in which they observed a drop in Prl levels in the second and third trimesters [22]. In contrast, a study conducted on non-pregnant women in Iran found a lower prevalence of T. gondii infections in patients with high Prl levels [25]. The same was observed in a study from India, in which they also found a lower prevalence of IgG seropositivity in non-pregnant women with high Prl levels [27]. On the other hand, a study showed an inhibitory effect of Prl on the replication of Toxoplasma in peripheral blood mononuclear cells of patients with hyperprolactinemia [26].
Furthermore, in a study executed on THP-1 cells pretreated with Prl (200 ng/mL), E2 (40 nM), and P4 (40 nM) and infected with T. gondii tachyzoites, in which the hormonal receptor expression (PrlR, ERα, and ERβ) and 17 cytokines were evaluated, it was observed that Prl did not alter the production of IL-12 or IL-1β, but increased IL-10, IL-4 and IL-13 and decreased the expression of ERα, Erβ, demonstrating the importance of Prl in the immune response against a Toxoplasma infection [16,17].
Previous studies suggest that Prl plays a fundamental role in the immune response against T. gondii infection. However, the decrease in Prl levels in seropositive patients in the third trimester of pregnancy, which was found in this study, is not completely clear and may be due to the modulation of stress responses during pregnancy.
With regards to the clinical features, 31.6% of patients had a history of miscarriage or stillborn, of which 36.8% were seropositive for anti-Toxoplasma IgG, lower than the 44.9% found in women with repeated miscarriage in 1995 [1,8].
Finally, E2 can play a dual role in T. gondii infection. It promotes infection by activating the parasite’s Tg-HSD gene and decreases inflammatory processes through the ERα receptor. Recombinant prolactin rhPRL could play a protective role by inhibiting parasite replication and modulating cytokine production TNF-α, IFNγ, and IL-12, which has been previously demonstrated. Progesterone has a protective and immunomodulatory role during pregnancy, protecting the fetus. The progesterone receptor (PGRMC) can regulate and promote the growth, proliferation, and differentiation of Toxoplasma. The T. gondii progesterone receptor membrane protein (TgPGRMC) can interact with E2 receptors ERα and ERβ. Progesterone can reduce parasite replication through GPER, decreasing the secretion of the parasite’s MIC2 protein while reducing its pathogenicity.
Future studies are necessary to understand other molecules and their mechanisms and signaling pathways that allow us to know the behavior of estradiol, prolactin, and progesterone in Toxoplasma infection during pregnancy.
5. Conclusions
E2 levels increased, without a relationship with the presence of anti-T. gondii antibodies, during pregnancy.
Progesterone is associated with high levels of IgG anti-Toxoplasma antibodies in the third trimester of gestation.
Prolactin levels in the second trimester decreased in seronegative women.
The hormones 17β-estradiol, progesterone, and prolactin may be immunomodulators in T. gondii infection during pregnancy.
Supplementary Materials
The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/cimb46060341/s1, Table S1: Sociodemographic variables and risk factors with anti-toxoplasma IgG antibodies.
Author Contributions
Conception and design of experiments, supervision, and project administration: M.d.l.L.G.-R.; performance of experiments: L.R.R.-P.; methodology: M.d.l.L.G.-R.; software: Y.G.L.R.; investigation: E.E.C.P.; funding acquisition: M.d.l.L.G.-R.; statistical analysis: M.d.l.L.G.-R. and Y.G.L.R.; writing of paper: E.E.C.P.; patients and clinical aspects: Y.G.L.R. All authors have read and agreed to the published version of the manuscript.
Funding
This work was partially supported by the Program to Support the Improvement of the Production Conditions of the SNI and SNCA Members (PRO-SNI 2022) and (PIN 2021 Number: 237086/2021 of the Universidad de Guadalajara.
Institutional Review Board Statement
This study was registered with number CI/033-22 and approved by the biosafety, research, and ethics committees of the University Center for Health Sciences at the University of Guadalajara.
Informed Consent Statement
All study participants and their tutors were informed about the purpose and procedures of this study and signed a written informed consent form.
Data Availability Statement
Data are contained within the article.
Acknowledgments
To the student of Eber Eduardo Soto Hernandez for her support in correcting this manuscript.
Conflicts of Interest
The authors declare no conflicts of interest.
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Figure 1.
The kinetics of anti-Toxoplasma IgG antibodies, with high levels in the first trimester and a tendency to decrease in the second and third trimesters of pregnancy. Concentration greater than 200 IU/mL corresponds to a patient with acute infection who was also positive for IgM (red line).
Figure 1.
The kinetics of anti-Toxoplasma IgG antibodies, with high levels in the first trimester and a tendency to decrease in the second and third trimesters of pregnancy. Concentration greater than 200 IU/mL corresponds to a patient with acute infection who was also positive for IgM (red line).
Figure 2.
Mean of levels of anti-Toxoplasma IgG antibodies, associated with hormone mean levels. The mean of P4 in seropositive women was higher than negatives p < 0.039 by pregnancy trimester.
Figure 2.
Mean of levels of anti-Toxoplasma IgG antibodies, associated with hormone mean levels. The mean of P4 in seropositive women was higher than negatives p < 0.039 by pregnancy trimester.
Figure 3.
Hormone concentration and association with positive and negative antibodies for anti-Toxoplasma. Progesterone had a sustained increase per trimester of gestation p < 0.39 while prolactin decreased in the third trimester p > 0.021.
Figure 3.
Hormone concentration and association with positive and negative antibodies for anti-Toxoplasma. Progesterone had a sustained increase per trimester of gestation p < 0.39 while prolactin decreased in the third trimester p > 0.021.
Figure 4.
The increase in hormone concentrations in all patients, with and without T. gondii infection (A) 17β-estradiol, (B) progesterone, and (C) prolactin, per trimester of gestation.First trimester (Purple Color), second trimester (Wine Color) and Third trimester (Blue Color).
Figure 4.
The increase in hormone concentrations in all patients, with and without T. gondii infection (A) 17β-estradiol, (B) progesterone, and (C) prolactin, per trimester of gestation.First trimester (Purple Color), second trimester (Wine Color) and Third trimester (Blue Color).
Table 1.
Quarterly anti-Toxoplasma antibodies and hormone mean.
| N | Minimum | Maximum | Mean | Standard Deviation | |
|---|---|---|---|---|---|
| 1T Toxoplasma IgG UI/mL | 52 | 0.86830 | 176.35000 | 27.11175 | 53.25078 |
| 2T Toxoplasma IgG UI/mL | 52 | 0.83000 | 219.33000 | 23.05660 | 49.10734 |
| 3T Toxoplasma IgG UI/mL | 52 | 0.83000 | 111.67000 | 12.96396 | 24.42573 |
| 1T Toxoplasma IgM UI/mL | 52 | 0.04477 | 1.43461 | 0.16810 | 0.21263 |
| 2T Toxoplasma IgM UI/mL | 52 | 0.01684 | 0.46863 | 0.14868 | 0.09057 |
| 3T Toxoplasma IgM UI/mL | 52 | 0.05472 | 0.48979 | 0.14377 | 0.09230 |
| ESTRADIOL 1T pg/mL | 52 | 376.72512 | 19,033.90000 | 3625.24431 | 3722.97799 |
| ESTRADIOL 2T pg/mL | 52 | 938.72444 | 27,051.50000 | 13,243.12995 | 7285.86553 |
| ESTRADIOL 3T pg/mL | 52 | 12,914.73 | 58,901.15 | 36,504.5008 | 12,114.67400 |
| PROLACTIN 1T ng/mL | 52 | 0.53000 | 540.98700 | 75.54135 | 76.42632 |
| PROLACTIN 2T ng/mL | 52 | 15.38000 | 584.96000 | 174.98144 | 134.67540 |
| PROLACTIN 3T ng/mL | 52 | 38.46000 | 625.00000 | 166.37818 | 120.15226 |
| PROGESTERONE 1T ng/mL | 52 | 10.791366 | 133.20000 | 55.14779 | 31.47740 |
| PROGESTERONE 2T ng/mL | 52 | 65.10791 | 555.29000 | 170.394048 | 110.82653 |
| PROGESTERONE 3T ng/mL | 52 | 129.439252 | 1187.83783 | 426.91970 | 275.42972 |
Table 2.
Hormonal levels associated with anti-Toxoplasma IgG antibodies during the first trimester of pregnancy.
Table 2.
Hormonal levels associated with anti-Toxoplasma IgG antibodies during the first trimester of pregnancy.
| Hormone TOXO | IgG | N | Mean | Standard Deviation | Standard Error | CI 95% Media | p | |
|---|---|---|---|---|---|---|---|---|
| Lower Bound | Upper Bound | |||||||
| ESTRADIOL | positive | 14 | 3941.24243 | 3326.45899 | 889.03356 | 2020.602 | 5861.882 | |
| negative | 38 | 3508.82395 | 3894.30121 | 631.73907 | 2228.798 | 4788.848 | 0.714 | |
| Total | 52 | 3625.24431 | 3722.97799 | 516.28415 | 2588.760 | 4661.728 | ||
| PROLACTIN | positive | 14 | 52.147164 | 32.48556 | 8.68213 | 33.390 | 70.903 | |
| negativo | 38 | 84.16026 | 86.00537 | 13.95191 | 55.891 | 112.429 | 0.183 | |
| Total | 52 | 75.54135 | 76.42632 | 10.59842 | 54.264 | 96.818 | ||
| PROGESTERONE | positive | 14 | 63.10866 | 33.85084 | 9.04701 | 43.563 | 82.653 | |
| negative | 38 | 52.214846 | 30.50103 | 4.94792 | 42.189 | 62.240 | 0.273 | |
| Total | 52 | 55.14779 | 31.47740 | 4.36513 | 46.384 | 63.911 | ||
Table 3.
Hormonal levels associated with anti-Toxoplasma IgG antibodies during the second trimester of pregnancy.
Table 3.
Hormonal levels associated with anti-Toxoplasma IgG antibodies during the second trimester of pregnancy.
| Hormone TOXO | IgG | N | Mean | Standard Deviation | Standard Error | CI 95% Media | p | |
|---|---|---|---|---|---|---|---|---|
| Lower Bound | Upper Bound | |||||||
| ESTRADIOL | positive | 14 | 15,622.66740 | 7179.86307 | 1918.89912 | 11,477.13788 | 19,768.19691 | |
| negative | 38 | 12,366.45826 | 7219.80052 | 1171.20630 | 9993.36888 | 14,739.54764 | 0.155 | |
| Total | 52 | 13,243.12995 | 7285.86553 | 1010.36776 | 11,214.73203 | 15,271.52787 | ||
| PROLACTIN | positive | 14 | 244.96568 | 170.40965 | 45.54389 | 146.57408 | 343.35728 | |
| negative | 38 | 149.19778 | 110.730559 | 17.96286 | 112.80155 | 185.59401 | 0.021 | |
| Total | 52 | 174.98144 | 134.67540 | 18.67611 | 137.48757 | 212.47532 | ||
| PROGESTERONE | positive | 14 | 219.17293 | 137.32029 | 36.70039 | 139.88656 | 298.45931 | |
| negative | 38 | 152.42287 | 95.25009 | 15.45160 | 121.11495 | 183.73080 | 0.053 | |
| Total | 52 | 170.39404 | 110.82653 | 15.36887 | 139.53974 | 201.24835 | ||
Table 4.
Hormonal levels associated with anti-Toxoplasma IgG antibodies during the third trimester of pregnancy.
Table 4.
Hormonal levels associated with anti-Toxoplasma IgG antibodies during the third trimester of pregnancy.
| Hormone TOXO | IgG | N | Mean | Standard Deviation | Standard Error | CI 95% Media | p | |
|---|---|---|---|---|---|---|---|---|
| Lower Bound | Upper Bound | |||||||
| ESTRADIOL | positive | 17 | 40,845.9224 | 13,959.58813 | 3385.69743 | 33,668.5644 | 48,023.2803 | |
| negative | 35 | 34,395.8103 | 10,697.80746 | 1808.25950 | 30,720.9848 | 38,070.6357 | 0.071 | |
| Total | 52 | 36,504.5008 | 12,114.67400 | 1680.00301 | 33,131.7540 | 39,877.2475 | ||
| PROLACTIN | positive | 17 | 155.89054 | 93.587113 | 22.69820 | 107.77249 | 204.00859 | |
| negative | 35 | 171.47218 | 132.10402 | 22.329655 | 126.092862 | 216.85150 | 0.665 | |
| Total | 52 | 166.378184 | 120.152262 | 16.66212 | 132.92758 | 199.828787839996270 | ||
| PROGESTERONE | positive | 17 | 539.56442 | 290.48655 | 70.45333 | 390.21001 | 688.91882 | |
| negative | 35 | 372.20655 | 254.27726 | 42.98070 | 284.85926 | 459.55385 | 0.039 | |
| Total | 52 | 426.91970 | 275.42972 | 38.195230 | 350.23958 | 503.59983 | ||
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Luna Rojas, Y.G.; Camarena Pulido, E.E.; Rodríguez-Pérez, L.R.; Galván-Ramírez, M.d.l.L. Follow-Up Study of 17-β Estradiol, Prolactin and Progesterone with the Kinetics and Prevalence of T. gondii Infection in Pregnant Women. Curr. Issues Mol. Biol. 2024, 46, 5701-5711. https://doi.org/10.3390/cimb46060341
AMA Style
Luna Rojas YG, Camarena Pulido EE, Rodríguez-Pérez LR, Galván-Ramírez MdlL. Follow-Up Study of 17-β Estradiol, Prolactin and Progesterone with the Kinetics and Prevalence of T. gondii Infection in Pregnant Women. Current Issues in Molecular Biology. 2024; 46(6):5701-5711. https://doi.org/10.3390/cimb46060341
Chicago/Turabian StyleLuna Rojas, Yithzel Guadalupe, Eva Elizabet Camarena Pulido, Laura Rocío Rodríguez-Pérez, and María de la Luz Galván-Ramírez. 2024. "Follow-Up Study of 17-β Estradiol, Prolactin and Progesterone with the Kinetics and Prevalence of T. gondii Infection in Pregnant Women" Current Issues in Molecular Biology 46, no. 6: 5701-5711. https://doi.org/10.3390/cimb46060341
APA StyleLuna Rojas, Y. G., Camarena Pulido, E. E., Rodríguez-Pérez, L. R., & Galván-Ramírez, M. d. l. L. (2024). Follow-Up Study of 17-β Estradiol, Prolactin and Progesterone with the Kinetics and Prevalence of T. gondii Infection in Pregnant Women. Current Issues in Molecular Biology, 46(6), 5701-5711. https://doi.org/10.3390/cimb46060341
