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雄激素诱导雄性化虹鳟鱼卵巢向精巢转分化过程中候选基因的表达谱分析

Expression profiling of candidate genes during ovary-to-testis trans-differentiation in rainbow trout masculinized by androgens.

作者信息

Baron Daniel, Houlgatte Rémi, Fostier Alexis, Guiguen Yann

机构信息

INRA, UR1037 SCRIBE, IFR140, Ouest-Genopole, Rennes, France.

出版信息

Gen Comp Endocrinol. 2008 Apr 1;156(2):369-78. doi: 10.1016/j.ygcen.2008.01.016. Epub 2008 Jan 29.

DOI:10.1016/j.ygcen.2008.01.016
PMID:18299129
Abstract

Fish gonadal phenotype is very sensitive to sex steroid and functional masculinizations can be obtained in most species using androgen treatments. To gain insight into the molecular effects of androgen-induced masculinization we characterized, in the rainbow trout, the gonadal expression profiles of 103 candidate genes involved in sex differentiation and early gametogenesis. The androgen treatment (11beta-hydroxyandrostenedione, 10 mg/kg of food for 3 months) was administered in a genetic all-female population. Gonads were sampled at different time points in genetic all-male and all-female control populations and in the androgen-treated group. Gene expression profiles were recorded by real-time RT-PCR and biological samples and gene expressions were compared using a global clustering analysis. This analysis revealed that masculinization with androgens acts firstly by repressing granulosa cell related genes, including genes involved in ovarian differentiation (foxl2a, fst, cyp19a1a), and subsequently by repressing genes important for early oogenesis (gdf9, bcl2lb, fancl, gcl, fshb, lhb, sox23, sox24, nup62 and vtgr). However, this masculinizing treatment did not induce a testicular differentiation similar to what was observed in the control male population. This was especially noticeable for many Leydig cell genes encoding proteins involved in steroidogenesis or its control (hsd3b1, star, cyp17a1, cyp11b2.1 and nr5a1b) that were down-regulated in the androgen-treated group. Concomitantly some Sertoli cells marker genes were up-regulated by the androgen treatment (sox9a.1, nr0b1, cldn11, dmrt1) whereas others were down-regulated (amh, sox9a.2), suggesting a partial differentiation of the Sertoli cell lineage. Overall, this suggests that the crucial step of this masculinization process is the de-differentiation of the granulosa cells.

摘要

鱼类性腺表型对性类固醇非常敏感,在大多数物种中使用雄激素处理可实现功能性雄性化。为深入了解雄激素诱导雄性化的分子效应,我们在虹鳟鱼中对参与性别分化和早期配子发生的103个候选基因的性腺表达谱进行了表征。雄激素处理(11β-羟基雄烯二酮,10毫克/千克饲料,持续3个月)应用于遗传全雌群体。在遗传全雄和全雌对照群体以及雄激素处理组的不同时间点采集性腺样本。通过实时RT-PCR记录基因表达谱,并使用全局聚类分析比较生物样本和基因表达。该分析表明,雄激素诱导的雄性化首先通过抑制颗粒细胞相关基因起作用,包括参与卵巢分化的基因(foxl2a、fst、cyp19a1a),随后通过抑制早期卵子发生重要的基因(gdf9、bcl2lb、fancl、gcl、fshb、lhb、sox23、sox24、nup62和vtgr)。然而,这种雄性化处理并未诱导出与对照雄性群体中观察到的类似的睾丸分化。对于许多编码参与类固醇生成或其调控的蛋白质的莱迪希细胞基因(hsd3b1、star、cyp17a1、cyp11b2.1和nr5a1b),在雄激素处理组中下调,这一点尤为明显。同时,一些支持细胞标记基因在雄激素处理下上调(sox9a.1、nr0b1、cldn11、dmrt1),而其他基因则下调(amh、sox9a.2),表明支持细胞谱系存在部分分化。总体而言,这表明该雄性化过程的关键步骤是颗粒细胞的去分化。

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