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父本附属性腺分泌物的缺失会干扰金黄地鼠胚胎中Igf2和Dlk1的表观遗传重编程及表达。

Absence of paternal accessory sex gland secretions disturbs epigenetic reprogramming and expression of Igf2 and Dlk1 in golden hamster embryos.

作者信息

Poon H K, Lee K H, Wong C L, O W S, Chow P H

机构信息

Department of Anatomy, Faculty of Medicine, The Chinese University of Hong Kong, Hong Kong SAR, China.

出版信息

Theriogenology. 2009 Jun;71(9):1367-80. doi: 10.1016/j.theriogenology.2008.12.016. Epub 2009 Feb 6.

Abstract

Accessory sex gland (ASG) secretion is known to exert an effect on sperm that is heritable in hamster embryos. We hypothesized that ASG secretion changes the sperm epigenome, which in turn is propagated in sired embryos. To test our hypothesis, we produced male hamsters that were devoid of either all ASG (TX) or only the ventral lobe of the prostate gland (VPX). A sham-operated control group (SH) was also established. These males were mated with normal females; uterine sperm, fertilized oocytes, and pre-implantation embryos were harvested from the females after mating. Epididymal sperm were collected at the end of experiments. Immunofluorescent staining was performed on these harvested specimens using antibodies against 5-methylcytosine, Dnmt1, Dnmt3a, Dnmt3b, protamine 1, protamine 2, and aectyl-H4K5. Expression of Igf2 and Dlk1 were analyzed by real-time RT PCR and in situ hybridization. We demonstrated that the DNA methylation pattern changed dynamically in SH, TX, and VPX fertilized oocytes. In VPX and TX embryos, DNA demethylation was slower and remethylation was delayed when compared with SH embryos. In addition, Dnmt3b expression was also abnormal. When sperm from VPX and TX males were exposed to whole ASG secretion in vivo, the resulting embryos all methylated normally. Immunofluorescent staining revealed that there was no difference in protamine packaging of uterine sperm from VPX and TX males. The staining also showed a lower level of acetyl-H4K5 expression in the male pronuclei of TX produced embryos. Furthermore, the VPX and TX embryos also expressed higher levels Igf2, and Dlk1. We concluded that interactions between ASG and sperm affected: (1) histone acetylation in male pronuclei; (2) DNA methylation in fertilized oocytes; and (3) Igf2 and Dlk1 expression embryos.

摘要

已知附属性腺(ASG)分泌物对精子有影响,这种影响在仓鼠胚胎中是可遗传的。我们假设ASG分泌物会改变精子表观基因组,进而在子代胚胎中传播。为了验证我们的假设,我们培育了完全没有所有附属性腺(TX)或仅没有前列腺腹叶(VPX)的雄性仓鼠。还设立了假手术对照组(SH)。这些雄性与正常雌性交配;交配后从雌性体内采集子宫内的精子、受精卵和植入前胚胎。实验结束时收集附睾精子。使用针对5-甲基胞嘧啶、Dnmt1、Dnmt3a、Dnmt3b、鱼精蛋白1、鱼精蛋白2和乙酰化-H4K5的抗体对这些采集的标本进行免疫荧光染色。通过实时RT-PCR和原位杂交分析Igf2和Dlk1的表达。我们证明,在SH、TX和VPX受精卵中,DNA甲基化模式动态变化。与SH胚胎相比,VPX和TX胚胎中的DNA去甲基化较慢,重新甲基化延迟。此外,Dnmt3b的表达也异常。当来自VPX和TX雄性的精子在体内暴露于整个ASG分泌物时,产生的胚胎均正常甲基化。免疫荧光染色显示,VPX和TX雄性子宫内精子的鱼精蛋白包装没有差异。染色还显示,TX产生的胚胎雄性原核中乙酰化-H4K5的表达水平较低。此外,VPX和TX胚胎中Igf2和Dlk1的表达水平也较高。我们得出结论,ASG与精子之间的相互作用影响:(1)雄性原核中的组蛋白乙酰化;(2)受精卵中的DNA甲基化;(3)胚胎中Igf2和Dlk1的表达。

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