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建立用于评估男性生殖毒性的体外测试系统。

Development of an in vitro test system for assessment of male, reproductive toxicity.

机构信息

Bradford School of Medical Sciences, School of Life Sciences, University of Bradford, Bradford, Richmond Road, West Yorkshire BD7 1DP, UK.

Bradford School of Medical Sciences, School of Life Sciences, University of Bradford, Bradford, Richmond Road, West Yorkshire BD7 1DP, UK.

出版信息

Toxicol Lett. 2014 Feb 10;225(1):86-91. doi: 10.1016/j.toxlet.2013.10.033. Epub 2013 Nov 12.

DOI:10.1016/j.toxlet.2013.10.033
PMID:24239781
Abstract

There is a need for improved reproductive toxicology assays that do not require large numbers of animals but are sensitive and informative. Therefore, Staput velocity-sedimentation separation followed by culture of specific mouse testicular cells was used as such a system. The specificity of separation was assessed using immunocytochemistry to identify spermatids, spermatocytes and spermatogonia. The efficacy of the system to detect toxicity was then evaluated by analysing the effects of hydrogen peroxide (H2O2) by the terminal uridine-deoxynucleotide end-labelling (TUNEL) assay to show the rate of apoptosis induced among the different types of germ cells. We found that 2 h of treatment at both 1 and 10 μM induced increases of over ∼10-fold in the percentage of apoptotic cells (p≤0.001), confirming that testicular germ cells are prone to apoptosis at very low concentrations of H2O2. It was also demonstrated for the first time for this compound that spermatogonia are significantly more susceptible than spermatocytes, which are more affected than spermatids. This reflects the proportion of actively dividing cells in these cell types, suggesting a mechanism for the differential sensitivity. The approach should thus form the basis of a useful test system for reproductive and genetic toxicology in the future.

摘要

需要改进生殖毒理学检测方法,这些方法不需要大量的动物,但需要具有敏感性和信息量。因此,采用了 Staput 速度沉降分离,然后培养特定的小鼠睾丸细胞,作为这样的系统。通过免疫细胞化学鉴定精子细胞、精母细胞和精原细胞来评估分离的特异性。然后,通过末端尿嘧啶脱氧核苷酸末端标记(TUNEL)测定分析过氧化氢(H2O2)的作用来评估该系统检测毒性的功效,以显示不同类型生殖细胞诱导的细胞凋亡率。我们发现,在 1 和 10 μM 下处理 2 小时,诱导凋亡细胞的百分比增加了约 10 倍以上(p≤0.001),证实了生殖细胞在非常低浓度的 H2O2 下容易发生凋亡。这也是首次证明该化合物对精原细胞的敏感性明显高于精母细胞,而精母细胞的敏感性又高于精子细胞。这反映了这些细胞类型中活跃分裂细胞的比例,提示了这种差异敏感性的机制。因此,该方法应该成为未来生殖和遗传毒理学有用的测试系统的基础。

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