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巨石斑鱼雌性向雄性性逆转过程中性别二态性标记基因Dmrt1和Foxl2的分子克隆与定量表达

Molecular cloning and quantitative expression of sexually dimorphic markers Dmrt1 and Foxl2 during female-to-male sex change in Epinephelus merra.

作者信息

Alam Mohammad Ashraful, Kobayashi Yasuhisa, Horiguchi Ryo, Hirai Toshiaki, Nakamura Masaru

机构信息

Sesoko Station, Tropical Biosphere Research Center, University of the Ryukyus, Sesoko 3422, Motobu, Okinawa 905-0227, Japan.

出版信息

Gen Comp Endocrinol. 2008 May 15;157(1):75-85. doi: 10.1016/j.ygcen.2008.03.018. Epub 2008 Mar 25.

Abstract

The honeycomb grouper (Epinephelus merra) is one of the smallest members of the Serranidae family and is often used to study protogynous sex change. To determine the role of the male-determining gene Dmrt1 and the ovarian-specific gene Foxl2 in sex change, we cloned these two markers from E. merra gonads by reverse transcription polymerase chain reaction (RT-PCR) and rapid amplification of cDNA ends (RACE). Two isoforms, Dmrt1a and Dmrt1b, resulted from alternative splicing in the coding region, causing the insertion of one glutamine residue in Dmrt1b. RT-PCR revealed that Dmrt1 was expressed only in the gonads, with higher levels in the testis than in the ovary. cDNA encoding Foxl2 was isolated from the ovary; Foxl2 was expressed extensively in the brain, pituitary, gonads, and gill, with its highest level in the ovary, indicating a potential role for Foxl2 in the brain-pituitary-gonad axis. Real-time quantitative RT-PCR analyses showed that Foxl2 mRNA expression was significantly downregulated from the late transitional phase to the completion of sex change. Conversely, Dmrt1 expression increased with the progression of spermatogenesis and continued until the formation of the testis. The expression profiles of these two sex-specific marker genes corresponded closely with the histological process of sex change. The down-regulation of Foxl2 most likely facilitates oocyte degeneration, whereas the up-regulation of Dmrt1 causes the proliferation of gonial germ cells into spermatogina and initiates sex change.

摘要

蜂巢石斑鱼(Epinephelus merra)是鮨科中最小的成员之一,常被用于研究雌性先熟的性别转变。为了确定雄性决定基因Dmrt1和卵巢特异性基因Foxl2在性别转变中的作用,我们通过逆转录聚合酶链反应(RT-PCR)和cDNA末端快速扩增(RACE)从蜂巢石斑鱼性腺中克隆了这两个标记。编码区的可变剪接产生了两种异构体,Dmrt1a和Dmrt1b,导致Dmrt1b中插入了一个谷氨酰胺残基。RT-PCR显示,Dmrt1仅在性腺中表达,在睾丸中的表达水平高于卵巢。从卵巢中分离出编码Foxl2的cDNA;Foxl2在脑、垂体、性腺和鳃中广泛表达,在卵巢中的表达水平最高,表明Foxl2在脑-垂体-性腺轴中具有潜在作用。实时定量RT-PCR分析表明,从晚期过渡阶段到性别转变完成,Foxl2 mRNA表达显著下调。相反,Dmrt1的表达随着精子发生的进展而增加,并持续到睾丸形成。这两个性别特异性标记基因的表达谱与性别转变的组织学过程密切相关。Foxl2的下调最有可能促进卵母细胞退化,而Dmrt1的上调导致生殖细胞增殖为精原细胞并启动性别转变。

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