Abstract

The mechanical method to isolate preantral follicle has been reported for many years. However, the culture systems in vitro are still unstable. The aim of this study was to analyze the effect of the culture system of mice preantral follicles on the follicular development in vitro. The results showed that the 96-well plate system was the most effective method for mice follicle development in vitro (volume change: 51.71%; survival rate: 89%, at day 4). Follicle-stimulating hormone (FSH) and Thyroid hormone (TH) are important for normal follicular development and dysregulation of hormones are related with impaired follicular development. To determine the effect of hormone on preantral follicular development, we cultured follicle with hormones in the 96-well plate culture system and found that FSH significantly increased preantral follicular growth on day 4. The FSH-induced growth action was markedly enhanced by T3 although T3 was ineffective alone. We also demonstrated by QRT-PCR that T3 significantly enhanced FSH-induced up-regulation of Xiap mRNA level. Meanwhile, Bad, cell death inducer, was markedly down-regulated by the combination of hormones. Moreover, QRT-PCR results were also consistent with protein regulation which detected by Western Blotting analysis. Taken together, the findings of the present study demonstrate that 96-well plate system is an effective method for preantral follicle development in vitro. Moreover, these results provide insights on the role of thyroid hormone in increasing FSH-induced preantral follicular development, which mediated by up-regulating Xiap and down-regulating Bad.

Highlights

  • Follicular development in ovary is highly extremely selective process in mammalian

  • We found that the combination of hormones up-regulated Xiap content and down-regulated Bad expression, which are the explanation of hormones promoted preantral follicle development

  • Follicles cultured in M1, M2 and M3 showed minimal growth, no significant difference in follicular growth were observed among three groups (P.0.05)

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Summary

Introduction

Follicular development in ovary is highly extremely selective process in mammalian. The destiny of major follicles is atresia. The transition from preantral to antral is the key stage during follicle development, which regulated by survival and death factors [1]. The fertilizable oocytes have been developed from mouse primordial and early preantral follicles in vitro [8,9,10], the follicle culture system for assaying the mechanism of preantral follicular development is still unstable. It is very important to develop FSH (follicle-stimulating hormone) free culture medium in preantral mouse follicle culture, which is used for analyzing the mechanism of factors affecting follicular development. In order to increase follicle survival rate in vitro, FSH is supplied in the culture medium. Since the culture systems with or without FSH are still unstable, it is necessary to develop new basic culture systems for preantral follicle growth without extra FSH

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