分子生物学标记BCL-2:白小鼠产前注射雌激素睾丸分析

R. T. Sulaimanova, A. Kvochko
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引用次数: 0

摘要

免疫组织化学研究是一种现代疾病诊断方法,用于实际兽医实践,以及在动物疾病的肿瘤和非肿瘤性质的鉴别诊断的科学发展。雌激素的产前影响导致成年生物的生殖系统紊乱,并伴随着后代睾丸和卵巢中类固醇依赖性癌症的平行生长。本研究的目的是在产前暴露于不同剂量的合成雌激素类似物Sinestrol时,对白种非纯种实验室小鼠后代睾丸中的Bcl-2标志物进行免疫组织化学分析。受精后,将怀孕雌鼠分为3组,1个完整组和2个实验组。完整组未受影响(n = 10)。第一实验组C-25 (n = 13)以2%油溶液形式注射雌激素药物Sinestrol,剂量为25 g/kg。第二实验组(n = 13)给予雌激素制剂Sinestrol 2%油溶液,剂量为40 mkg/kg。当后代达到性成熟时,他们被从实验中移除。对子代睾丸石蜡切片进行标准形态学研究免疫组化分析,测定子代雄性腺体细胞成分指标:精原细胞、精母细胞、精潮细胞、精子和间质细胞中凋亡抑制剂Bcl-2的标记物。暴露于合成药物Sinestrol 25和40 g/kg剂量时,Bcl-2标记物的表达表明,精原细胞中阳性染色细胞的数量分别比完整组增加了8.6%和9.4%。完整组与实验组C-25、C-40比较,精母细胞和精子中Bcl-2标记物的表达无差异,精母细胞中阳性染色细胞略有增加。Bcl-2标志物在间质细胞中的表达率在实验组c25和c40中分别下降了56.0% (P < 0.05)和60.0% (P < 0.05)。在胎儿腺体起始阶段给予合成雌激素类似物辛雌醇导致成年后睾丸形态受损。实验组C-25和C-40间质细胞Bcl-2标记物表达指数下降,导致细胞凋亡死亡,该细胞负责雄性性激素睾酮的产生。该结果可用于产前选择合成雌激素类似物辛雌醇的最佳剂量。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Molecular biological marker BCL-2: testis analysis in prenatal injection of estrogen to white laboratory mice
Immunohistochemical study is one of the modern methods of disease diagnostics used in practical veterinary practice, as well as in scientific developments in differential diagnostics of animal diseases of tumour and non-tumour nature. Prenatal influence of estrogens results in reproductive system disorders in an adult organism which is accompanied by parallel growth of steroid dependent cancers of the offspring: testicles and ovaries. The aim of the study was to perform immunohistochemical analysis of Bcl-2 marker during prenatal exposure to different doses of the synthetic estrogen analogue Sinestrol in the testes of the offspring of white non-pedigreed laboratory mice. After fertilization, the pregnant females were divided into 3 groups, one intact and two experimental groups. The intact group was unaffected (n = 10). The first experimental group, C-25 (n = 13), was injected with the estrogen drug Sinestrol in the form of a 2 % oil solution at a dose of 25 g/kg. The second experimental group (n = 13) was given the estrogen preparation Sinestrol in the form of 2 % oil solution in a dose of 40 mkg/kg. When the offspring reached sexual maturity, they were removed from the experiment. Immunohistochemical analysis was carried out on sections from paraffin blocks of testes of progeny intended for standard morphological study, the marker of apoptosis inhibitor Bcl-2 was determined on indices of cellular elements of male glands of progeny: spermatogonia, spermatocytes, sperm-tides, spermatozoa and Leydig cells. Expression of Bcl-2 marker upon exposure to the synthetic drug Sinestrol at doses of 25 and 40 g/kg showed that the number of positively stained cells in spermatogonia increased by 8.6 and 9.4 % respectively compared to the intact group. When the intact group was compared with experimental groups C-25 and C-40, the expression of Bcl-2 marker in spermatocyte cells and spermatozoa showed no difference, a slight increase in positively stained cells in spermatids was observed. Bcl-2 marker expression rate in experimental groups C 25 and C-40 decreased in Leydig cells by 56.0 (P 0.05) and 60.0 % (P 0.05), respectively. Administration of the synthetic estrogen analogue Sinestrol during fetal gland initiation resulted in impaired morphology in the testes in adulthood. The expression index of Bcl-2 marker in experimental groups C-25 and C-40 decreased in Leydig cells, resulting in apoptotic cell death, which is responsible for production of male sex hormone testosterone. The results can be used to select optimal doses of the synthetic estrogen analogue Sinestrol in the prenatal period.
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