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李广丽, 邓思平, 王文达, 孙晶, 吴天利, 师尚丽, 朱春华. 性类固醇激素对胡子鲇性分化的影响[J]. 水生生物学报, 2013, 37(6): 1020-1027. DOI: 10.7541/2013.136
引用本文: 李广丽, 邓思平, 王文达, 孙晶, 吴天利, 师尚丽, 朱春华. 性类固醇激素对胡子鲇性分化的影响[J]. 水生生物学报, 2013, 37(6): 1020-1027. DOI: 10.7541/2013.136
LI Guang-li, DENG Si-ping, WANG Wen-da, SUN Jing, WU Tian-li, SHI Shang-li, ZHU Chun-hua. EFFECTS OF SEX STEROID HORMONES ON SEX DIFFERENTIATION OF CLARIAS FUSCUS[J]. ACTA HYDROBIOLOGICA SINICA, 2013, 37(6): 1020-1027. DOI: 10.7541/2013.136
Citation: LI Guang-li, DENG Si-ping, WANG Wen-da, SUN Jing, WU Tian-li, SHI Shang-li, ZHU Chun-hua. EFFECTS OF SEX STEROID HORMONES ON SEX DIFFERENTIATION OF CLARIAS FUSCUS[J]. ACTA HYDROBIOLOGICA SINICA, 2013, 37(6): 1020-1027. DOI: 10.7541/2013.136

性类固醇激素对胡子鲇性分化的影响

EFFECTS OF SEX STEROID HORMONES ON SEX DIFFERENTIATION OF CLARIAS FUSCUS

  • 摘要: 研究采用组织学和荧光实时定量PCR方法,检测17-甲基睾酮(17-MT)和17-雌二醇(17-E2)对胡子鲇(Clarias fuscus)性腺组织学、性别比率以及性分化前后脑型芳香化酶基因(Cyp19a1b)和翼状螺旋/叉头转录因子2(Foxl2)基因表达的影响。结果表明:在出膜后230日龄,17-MT (50、100和200 g/L)浸浴、17-E2(100、200和300 g/g)投喂处理对成活率无显著影响,但中、高剂量(100和200 g/L)17-MT显著抑制卵巢发育,促进精巢发育,卵巢腔出现时间分别推迟4d和6d,初级卵母细胞出现时间分别推迟8d和9d,而初级精母细胞出现时间则分别提前3d和5d,且雄性率分别达70%和76%,显著高于50 g/L组和对照组(P0.05)。相反,中、高剂量17-E2(200和300 g/g)处理使卵巢腔出现时间分别提前2d和3d,初级卵母细胞出现时间分别提前1d和3d,初级精母细胞出现时间分别推迟3d和7d,而雌性率分别达74%和78%,显著高于100 g/g组和对照组(P0.05)。此外,在性腺分化期,17a-MT促进Cyp19a1b但抑制Foxl2的表达,而17-E2促进Cyp19a1b和 Foxl2的表达。结果显示Cyp19a1b不是引起胡子鲇性分化的直接因素,但可能通过下丘脑-垂体-性腺轴对胡子鲇性分化过程产生间接影响;而Foxl2直接参与胡子鲇的性分化,即17a-MT和17-E2分别通过抑制和促进Foxl2的表达来影响雌激素的生物合成,从而调控胡子鲇性分化的方向。

     

    Abstract: Clarias fuscus, a common freshwater fish in China, was selected as our experiment material. Two-day juvenile C. fuscus was divided into two groups. They were immersed in different doses of 17-methyltestosterone (50, 100, and 200 g/L 17-MT) or fed with 17-estradiol (100, 200, and 300 g/g 17-E2) for 30 days. Effects of 17-MT and 17-E2 on survival rate, sex ratio, gonad histology, and Foxl2 and Cyp19a1b expressions were examined by morphologic observation, histology and Real time fluorescent quantitative PCR during its period of sex differentiation (230d after hatching). The results showed that 17-MT and 17-E2 had no influence on survival rate but affected sex ratio and the time of gonadal differentiation. Doses of 17-MT at 100 and 200 g/L produced more males (70% and 76%, respectively) than 50 g/L 17-MT (54%) did (P0.05), but no significant difference in sex ratio was observed between the 50 g/L 17-MT treated group and the control group (56%). In addition, the former accelerated the occurrence of primary spermocytes for three and five days, but deferred that of ovarian cavity for four and six days, and primary oocytes for eight and nine days, respectively. In contrast, doses of 17-E2 at 200 and 300 g/g produced more males (74% and 78%, respectively) than the control group (P0.05), but no significant difference in sex ratio was observed between the 100 g/g 17-E2 treated group (66%) and the control group (56%). Dose of 17-E2 at 200 and 300 g/g accelerated the occurrence of ovarian cavity for two and three days, and primary oocytes for one and three days, respectively, but deferred that of primary spermatocytes for three and seven days. The expressions of Foxl2 and Cyp19a1b showed that dose of 200 g/L 17-MT increased the expression of Cyp19a1b but inhibited that of Foxl2.However, dose of 300g/g 17-E2 increased the expression both of Cyp19a1band Foxl2.The results suggested that Foxl2 but not Cyp19a1b involved in mediating sex differentiation directly in C. fuscus, and 17-MT inhibited but 17-E2 promoted the expressions of Foxl2 toinfluence the estrogen biosynthesis, which controlled the sex differentiation. However, Cyp19a1b played an indirect role on sex differentiation by acting on the hypothalamic-pituitary-gonadal axis.

     

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