RESUMEN
This study was performed to examine the effects of various macromolecules in in vitro growth (IVG) media on the growth, maturation, and parthenogenesis (PA) of pig oocytes derived from small antral follicles (SAF). Immature oocytes were cultured for two days in IVG medium supplemented with 10% (v/v) fetal bovine serum (FBS), 10% (v/v) pig follicular fluid (PFF), 0.4% (w/v) bovine serum albumin (BSA), or 0.1% (w/v) polyvinyl alcohol (PVA) and then maintained for 44 h for maturation. After IVG, the mean diameters of the SAF treated with FBS, PVA, and no IVG-MAF (113.0–114.8 µm) were significantly larger than that of no IVG-SAF (111.8 µm). The proportion of metaphase II oocytes was higher in PFF (73.6%) than in BSA (43.5%) and PVA (53.7%) but similar to that in the FBS treatment (61.5%). FBS and PFF increased cumulus expansion significantly compared to PVA and BSA while the intraoocyte glutathione content was not influenced by the macromolecules. Blastocyst formation of PA oocytes treated with FBS (51.8%), PFF (50.4%), and PVA (45.2%) was significantly higher than that of the BSA-treated oocytes (20.6%). These results show that the PFF and FBS treatments during IVG improved the growth, maturation, and embryonic development of SAF.
Asunto(s)
Femenino , Embarazo , Blastocisto , Desarrollo Embrionario , Líquido Folicular , Glutatión , Técnicas In Vitro , Metafase , Oocitos , Partenogénesis , Alcohol Polivinílico , Albúmina Sérica BovinaRESUMEN
This study investigated the levels of messenger ribonucleic acids (mRNA) for inhibin-ßA subunit in goat primordial, primary and secondary follicles, as well as in cumulus-oocyte complexes (COCs) and mural granulosa / theca cells of antral follicles. The effects of activin-A (100ng mL-1) and/or follicle stimulating hormone (FSH, 50ng mL-1) on growth and expression of mRNA for activin-A and FSH receptor (FSH-R) in secondary follicles cultured for six days were evaluated. The data showed that the expression of inhibin-ßA is lower in secondary follicles than in primary follicles and is higher in large antral follicles than in small antral follicles. After culture, activin-A and/or FSH promoted growth of secondary follicles, while FSH increased the levels of mRNA for inhibin-ßA, and activin-A increased the levels of FSH-R mRNA. In conclusion, mRNA for inhibin-ßA is expressed at different levels in pre-antral and antral follicles and activin-A acts as a stimulator of the FSH-R expression in goat follicles. On its turn, the expression of inhibin-ßA is stimulated by FSH, which together with activin-A promotes secondary follicle growth in-vitro.
Este estudo investigou os níveis de ácidos ribonucleicos (RNAm) para a subunidade ßA da inibina em folículos primordiais, primários e secundários caprinos, bem como em complexos cumulus-oócitos (CCOs) e células da granulosa mural/teca de folículos antrais. Além disso, avaliaram-se os efeitos da ativina-A (100ng mL-1) e/ou hormônio folículo estimulante (FSH, 50ng mL-1) sobre o crescimento e a expressão do RNAm para inibina-ßA e receptores de FSH (FSH-R) em folículos secundários cultivados por seis dias. Os dados mostraram que a expressão de inibina-ßA é menor em folículos secundários do que em folículos primários e é maior em grandes folículos antrais que nos pequenos folículos antrais. Após o cultivo, ativina-A e/ou FSH promoveram o crescimento de folículos secundários. Enquanto o FSH aumentou os níveis de RNAm para inibina-ßA, a ativina-A aumentou os níveis de RNAm para FSH-R. Em conclusão, a inibina-ßA é expressa em diferentes níveis em folículos pré-antrais e antrais e a ativina-A atua como um estimulador da expressão de FSH-R em folículos caprinos. Por sua vez, a expressão de inibina-ßA é estimulada pelo FSH, que, juntamente com ativina, promove o crescimento de folículos secundários in vitro.
RESUMEN
The sustainability and production of collared peccary (Pecari tajacu) has been studied in the last few years; however, further information on its reproduction is necessary for breeding systems success. Understanding folliculogenesis aspects will contribute to effective reproductive biotechniques, which are useful in the preservation and production of wildlife. The aim of this study was to evaluate the ovarian folliculogenesis in collared peccary. Ovaries from six adult females of collared peccary were obtained through ovariectomy and analyzed. These were fixed in aqueous Bouin’s solution and sectioned into 7μm slices, stained with hematoxilin-eosin and analyzed by light microscopy. The number of pre-antral and antral follicles per ovary was estimated using the Fractionator Method. The follicles, oocytes and oocyte nuclei were measured using an ocular micrometer. Results showed that the length, width, thickness, weight, and the gross anatomy of the right and left ovaries were not significantly different. However, the mean number of corpora lutea was different between the phases of the estrous cycle (p<0.05), with the highest mean in the luteal phase. Primordial follicles were found in the cortex; the oocytes were enveloped by a single layer of flattened follicular cells. In the primary follicles, proliferation of the follicular cells gave rise to cuboidal cells (granulosa cells). The secondary follicle was characterized by two or more concentric layers of cuboidal cells (granulosa), beginning of antrum formation, and the presence of pellucid zone and theca cells. Antral follicles were characterized by a central cavity (antrum), the presence of cumulus oophorus and theca layers (interna and externa). In the right ovary, the values of the primordial and primary follicles were similar, but significantly different from the secondary ones (p<0.05). In the left ovary, significant differences were observed between all follicles in the follicular phase (p<0.05); the mean number of primordial and primary follicles was similar in the luteal phase. The mean number of pre-antral follicles and antral follicles in the follicular phase was higher in the left ovary (p<0.05). The mean number of antral follicles in the luteal phase was similar in both ovaries. We also found significant differences in mean diameter of preantral follicles, oocyte, granulosa layer and oocyte nucleus during the estrous cycle. In the antral follicles a significant difference was observed only in follicular diameter (p<0.05). The predominance of active primordial and primary follicles was found in both phases; otherwise the secondary follicles and antral follicles showed a high degree of degeneration. The results obtained in the present work will strengthen the development of biotechnology programs to improve the productive potential and conservation of the collared peccary.
La sustentabilidad y la producción de pecarí de collar (Pecari tajacu) han sido estudiados en los últimos años, sin embargo, más información sobre su reproducción es necesaria para el éxito de los sistemas de crianza . La comprensión de los aspectos relacionados con la foliculogénesis contribuirá con la aplicación de biotécnicas de reproducción, las cuales son útiles en la preservación y la producción de la vida silvestre. El objetivo de este estudio fue obtener datos sobre la población folicular del ovario de pecarí de collar. En relación con la población folicular en el ovario derecho, los valores de los folículos primordiales y primarios fueron similares, pero se observó que había una diferencia significativa (p<0.05) con el secundario. En el ovario izquierdo, la fase folicular presentó diferencias significativas (p<0.05) entre todos los folículos, y en la fase lútea el número medio de folículos primordiales y primarios fueron similares. Ahora bien, con respecto a la población de folículos antrales, en la fase folicular, se observaron diferencias significativas entre los ovarios (p<0.05), y de forma similar en la fase lútea. También se encontraron diferencias significativas en el diámetro medio de los folículos preantrales, oocitos, la capa granulosa y el núcleo del oocito durante las fases del ciclo estral. Asimismo, en los folículos antrales se observó diferencia estadísticamente significativa (p<0.05) en el diámetro folicular. En ambas fases del ciclo estral, se encontró el predominio de folículos primordiales y primarios en desarrollo, por otro lado, los folículos secundarios y los folículos antrales mostraron un alto grado de degeneración. Los resultados aquí presentes son necesarios para el desarrollo de los programas de mejoramiento y conservación.
Asunto(s)
Animales , Femenino , Artiodáctilos/anatomía & histología , Folículo Ovárico/anatomía & histología , Artiodáctilos/fisiología , Ciclo Estral/fisiología , Fase Folicular/fisiología , Fase Luteínica/fisiología , Folículo Ovárico/fisiologíaRESUMEN
Objetivo: Comparar as curvas padrões de decréscimo da reserva ovariana considerando a dosagem do hormônio folículo estimulante (FSH) e a contagem dos folículos antrais (CFA). Método: Estudo transversal prospectivo de pacientes atendidas no Centro de Reprodução Fêmina no período de 01/03/2010 a 31/08/2010. As pacientes foram submetidas à ultrassonografia transvaginal e à dosagem do FSH do 2º ao 4º dia da menstruação. Foram incluídas pacientes de 21 a 44 anos, com ciclos regulares, dois ovários íntegros, nenhuma evidência de endocrinopatias, que não recebiam medicamentos há 6 meses, e que assinaram o consentimento. Foram excluídas as tabagistas, portadoras de galactosemia, cistos ovarianos, com antecedente de hepatopatia, cirurgia ginecológico-ovariana, tratamento com quimioterapia ou radioterapia. O teste utilizado foi o coeficiente de correlação de Pearson. Resultados: Sessenta e oito pacientes com idade entre 22 e 44 anos foram incluídas. O fator masculino foi a principal etiologia da infertilidade, contribuindo com 41% dos casos. A correlação entre a dosagem do FSH e a CFA foi fraca (r=-0,269) e o teste de Pearsonfoi estatisticamente signifi cante (p=0,026). Conclusão: A correlação entre a contagem dos folículos antrais e a dosagem sérica do hormônio folículo estimulante foi fraca e estatisticamente signifi cante.
Objective: To compare the curves patterns of ovarian reserve decline taking into account the follicle stimulating hormone measurement (FSH) and the antral follicles count (AFC). Methods: Prospective transversal study of patients attended at Fêmina Reproduction Center from March 2010 to August 2010. The patients were submitted to transvaginal ultrasonography and had FSH measurement from days 2 to 4 of their period. Patients included were the ones who were 21 to 44 years old, with regular menses, two healthy ovaries, without any evidence of endocrinopathies, that were not taking medicines for 6 months, and signed the consent. Patients excluded: smokers, with galactosemia or ovarian cysts, with antecedents of hepatopathies, gynecological ovarian surgeries or were treated with chemotherapy or x-ray. Pearsons correlation coefficient was used to analyze the data. Results: Sixty-eight patients were included in the trial, age ranged from 22 to 44 years old. The male factor was the main etiology of infertility, contributing with 41% of the cases. The correlation between FSH measurement and AFC was weak (r=-0,269) and Pearson test was statistically signifi cant (p=0,026). Conclusions: The correlation between the antral follicles count and the serum dosage of FSH was weak and statistically signifi cant.
Asunto(s)
Humanos , Femenino , Adulto , Hormona Folículo Estimulante , Infertilidad/etiología , Biomarcadores , Técnicas ReproductivasRESUMEN
OBJECTIVE: This present study was conducted to examine the effects on in vitro growth of pre-antral mouse follicles by thecal-stromal cells attached to around the follicular membrane in culture medium without hormones. METHODS: Pre-antral follicles (100-130 micro meter) used in our studies were isolated mechanically by fine 30 G needles attached to 1 ml insulin syringe from mice ovaries of 20-25 days old female ICR strain. Isolated pre-antral follicles were divided into three groups by attached status of thecal-stromal cell layers to follicular membrane. Follicular Initial diameters of group I was 112.5 (mean) +/- 6.2 (SD) micro meter (n=31), group II was 112.8 +/- 7.8 micro meter (n=23), and group III was 115.1 +/- 6.5 micro meter (n=27). Divided pre-antral follicles were washed in fresh Ham's F-10 medium and cultured in 20 micro liter droplets of DMEM with glutamine, glucose and pyruvate under mineral oil on the 60 mm culture dish. All experimental media were supplemented with 10% FBS without hormones. Media were exchanged wholly by fresh media every 2 days in culture. Diameters of intrafollicular oocytes and cultured pre-antral follicles were measured using an precalibrated cross ocular micrometer at X200 every day during 6 days in vitro culture. Results were considered statistically significant when p value was less than 0.05 using Student's t-test. RESULTS: The mean and standard deviation (SD) of initial diameters of pre-antral follicles was 113.5 +/- 2.2 micro meter in three groups. Follicular growth rate of group III was significantly (p<0.05) higher in whole culture periods than group I and group II. Rate of follicular growth between group I and group II were not significant difference in culture for 1 to 3 days. However, group II was significantly higher than group I in culture for 4 days. Diameters of grown follicles for 6 days was 155.2 +/- 18.7 micro meter, 196.9 +/- 24.1 micro meter and 284.2 +/- 47.6 micro meter in group I, group II and group III, respectively. Growth rate of intrafollicular oocytes between three groups were not difference and revealed to continuous growth patterns in whole culture periods. Follicular diameter after culture for 7 days were not measured because of disruption of follicular structure or outgrowth of granulosa cells. CONCLUSION: Pre-antral follicles were grown very well in DMEM medium without hormones. Thecal- stromal cells attached to the surface of follicular membrane has acted effectively in vitro growth of follicles.