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Does Rbmy have a role in sperm development in mice?

机译:Rbmy是否在小鼠精子发育中起作用?

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The Yd1 deletion in mice removes most of the multi-copy Rbmy gene cluster that is located adjacent to the centromere on the Y short arm (Yp). XYd1 mice develop as females because Sry is inactivated, probably because it is now juxtaposed to centromeric heterochromatin. We have previously produced XYd1Sry transgenic males and found that they have a substantially increased frequency of abnormal sperm. Staining of testis sections with a polyclonal anti-RBMY antibody appeared to show a marked decrease of RBMY protein in the spermatids of XYd1Sry males compared to control males, which led us to suggest that this may be responsible for the increase in sperm anomalies. In the current study we sought to determine whether augmenting Rbmy expression specifically in the spermatids of XYd1Sry males would ameliorate the sperm defects. An expressing Rbmy transgene driven by the spermatid-specific mouse protamine 1 promotor (mP1Rbmy) was therefore introduced into XYd1Sry males. This failed to reduce the frequency of abnormal sperm. In the course of this study, a new RBMY antibody was generated that, in contrast to the original antibody, failed to detect RBMY in spermatid stages by immunostaining. The lack of RBMY was confirmed by western blotting of lysates from purified round spermatids and elongating spermatids. The implications of these results for the proposed role for RBMY in sperm development are discussed.
机译:小鼠中的Yd1缺失可去除大部分与Y短臂(Yp)着丝粒相邻的多拷贝Rbmy基因簇。 XYd1小鼠发育成雌性,因为Sry被灭活,可能是因为它现在与着丝粒异染色质并列。我们以前已经生产了XYd1Sry转基因雄性,发现它们的异常精子发生频率大大增加。用多克隆抗RBMY抗体染色睾丸切片似乎显示XYd1Sry雄性精子中的RBMY蛋白与对照雄性相比明显减少,这使我们建议这可能是精子异常增加的原因。在当前的研究中,我们试图确定增强XYd1Sry雄性精子中Rbmy的表达是否会改善精子缺陷。因此,将由精子特异性小鼠鱼精蛋白1启动子(mP1Rbmy)驱动的表达Rbmy转基因引入XYd1Sry雄性。这未能减少精子异常的频率。在这项研究过程中,产生了一种新的RBMY抗体,与原始抗体相反,该抗体无法通过免疫染色检测精子期的RBMY。通过纯化的圆形精子和延伸精子的裂解物的蛋白质印迹法证实了RBMY的缺乏。讨论了这些结果对RBMY在精子发育中作用的建议意义。

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