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新生雄性大鼠暴露于强效和弱效(环境)雌激素对青春期精子发生的比较影响及其与成年睾丸大小和生育能力的关系:低雌激素水平具有刺激作用的证据

Comparative effects of neonatal exposure of male rats to potent and weak (environmental) estrogens on spermatogenesis at puberty and the relationship to adult testis size and fertility: evidence for stimulatory effects of low estrogen levels.

作者信息

Atanassova N, McKinnell C, Turner K J, Walker M, Fisher J S, Morley M, Millar M R, Groome N P, Sharpe R M

机构信息

Medical Research Council Human Reproductive Sciences Unit, Center for Reproductive Biology, Edinburgh, Scotland, United Kingdom.

出版信息

Endocrinology. 2000 Oct;141(10):3898-907. doi: 10.1210/endo.141.10.7723.

DOI:10.1210/endo.141.10.7723
PMID:11014247
Abstract

This study investigated whether neonatal exposure of male rats to estrogenic compounds altered pubertal spermatogenesis (days 18 and 25) and whether the changes observed resulted in long-term changes in testis size, mating, or fertility (days 90-100). Rats were treated neonatally with a range of doses (0.01-10 microg) of diethylstilbestrol (DES; administered on alternate days from days 2-12), a high dose of octylphenol (OP; 2 mg administered daily from days 2-12) or bisphenol A (Bis-A; 0.5 mg administered daily from days 2-12), or vehicle, while maintained on a standard soy-containing diet. The effect on the same parameters of rearing control animals on a soy-free diet was also assessed as was the effect of administering such animals genistein (4 mg/kg/day daily from days 2-18). Testis weight, seminiferous tubule lumen formation, the germ cell apoptotic index (apoptotic/viable germ cell nuclear volume), and spermatocyte nuclear volume per unit Sertoli cell nuclear volume were used to characterize pubertal spermatogenesis. Compared with (soy-fed) controls, DES administration caused dose-dependent retardation of pubertal spermatogenesis on day 18, as evidenced by decreases in testis weight, lumen formation, and spermatocyte nuclear volume per unit Sertoli cell and elevation of the germ cell apoptotic index. However, the two lowest doses of DES (0.1 and 0.01 microg) significantly increased spermatocyte nuclear volume per unit Sertoli cell. Similarly, treatment with either OP or Bis-A significantly advanced this and some of the other aspects of pubertal spermatogenesis. Maintenance of control animals on a soy-free diet also significantly advanced lumen formation and spermatocyte nuclear volume per unit Sertoli cell compared with controls fed a soy-containing diet. Administration of genistein reversed the stimulatory effects of a soy-free diet and significantly retarded most measures of pubertal spermatogenesis. In general, plasma FSH levels in the treatment groups changed in parallel to the spermatogenic changes (reduced when pubertal spermatogenesis retarded, increased when pubertal spermatogenesis advanced). By day 25, although the changes in FSH levels largely persisted, all of the stimulatory effects on spermatogenesis seen on day 18 in the various treatment groups were no longer evident. In adulthood, testis weight was decreased dose dependently in rats treated neonatally with DES, but only the lowest dose group (0.01 microg) showed evidence of mating (3 of 6) and normal fertility (3 litters). Animals treated neonatally with OP or Bis-A had normal or increased (Bis-A) testis weights and exhibited reasonably normal mating/fertility. Animals fed a soy-free diet had significantly larger testes than controls fed a soy-containing diet, and this difference was confirmed in a much larger study of more than 24 litters, which also showed a significant decrease in plasma FSH levels and a significant increase in body weight in the males kept on a soy-free diet. Neonatal treatment with genistein did not alter adult testis weight, and although most males exhibited normal mating and fertility, a minority did not mate or were infertile. It is concluded that 1) neonatal exposure of rats to low levels of estrogens can advance the first wave of spermatogenesis at puberty, although it is unclear whether this is due to direct effects of the estrogen or to associated elevation of FSH levels; 2) the effect of high doses of OP and Bis-A on these processes is essentially benign; and 3) the presence or absence of soy or genistein in the diet has significant short-term (pubertal spermatogenesis) and long-term (body weight, testis size, FSH levels, and possibly mating) effects on males.

摘要

本研究调查了雄性大鼠在新生儿期暴露于雌激素化合物是否会改变青春期精子发生(第18天和第25天),以及所观察到的变化是否会导致睾丸大小、交配或生育能力的长期变化(第90 - 100天)。大鼠在新生儿期接受一系列剂量(0.01 - 10微克)的己烯雌酚(DES;从第2天至第12天隔日给药)、高剂量的辛基酚(OP;从第2天至第12天每天给药2毫克)或双酚A(Bis - A;从第2天至第12天每天给药0.5毫克)或赋形剂处理,同时维持标准的含大豆饮食。还评估了在无大豆饮食中饲养对照动物对相同参数的影响,以及给这些动物施用染料木黄酮(从第2天至第18天每天4毫克/千克)的效果。睾丸重量、生精小管管腔形成、生殖细胞凋亡指数(凋亡/存活生殖细胞核体积)以及每单位支持细胞核体积的精母细胞核体积用于表征青春期精子发生。与(喂食大豆的)对照组相比,DES给药导致第18天青春期精子发生呈剂量依赖性延迟,表现为睾丸重量、管腔形成以及每单位支持细胞的精母细胞核体积减小,生殖细胞凋亡指数升高。然而,DES的两个最低剂量(0.1和0.01微克)显著增加了每单位支持细胞的精母细胞核体积。同样,用OP或Bis - A处理显著提前了青春期精子发生的这一过程以及其他一些方面。与喂食含大豆饮食的对照组相比,在无大豆饮食中饲养对照动物也显著提前了管腔形成以及每单位支持细胞的精母细胞核体积。施用染料木黄酮逆转了无大豆饮食的刺激作用,并显著延迟了青春期精子发生的大多数指标。一般来说,治疗组的血浆促卵泡激素(FSH)水平与精子发生变化平行(青春期精子发生延迟时降低,青春期精子发生提前时升高)。到第25天,尽管FSH水平的变化大多持续存在,但在第18天各治疗组中观察到的对精子发生的所有刺激作用不再明显。在成年期,新生儿期用DES处理的大鼠睾丸重量呈剂量依赖性降低,但只有最低剂量组(0.01微克)显示有交配迹象(6只中有3只)和正常生育能力(3窝)。新生儿期用OP或Bis - A处理的动物睾丸重量正常或增加(Bis - A组)且表现出相当正常的交配/生育能力。喂食无大豆饮食的动物睾丸明显大于喂食含大豆饮食的对照组,并且在一项对超过24窝的更大规模研究中证实了这一差异,该研究还显示无大豆饮食饲养的雄性大鼠血浆FSH水平显著降低,体重显著增加。新生儿期用染料木黄酮处理未改变成年期睾丸重量,并且尽管大多数雄性表现出正常的交配和生育能力,但少数未交配或不育。结论是:1)大鼠在新生儿期暴露于低水平雌激素可提前青春期精子发生的第一波,尽管尚不清楚这是由于雌激素的直接作用还是FSH水平的相关升高;2)高剂量的OP和Bis - A对这些过程的影响基本是良性的;3)饮食中大豆或染料木黄酮的存在与否对雄性有显著的短期(青春期精子发生)和长期(体重、睾丸大小、FSH水平以及可能的交配)影响。

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