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聚(ADP - 核糖)稳态的破坏会影响小鼠精子发生和精子染色质完整性。

Disruption of poly(ADP-ribose) homeostasis affects spermiogenesis and sperm chromatin integrity in mice.

作者信息

Meyer-Ficca Mirella L, Lonchar Julia, Credidio Christine, Ihara Motomasa, Li Yun, Wang Zhao-Qi, Meyer Ralph G

机构信息

Department of Animal Biology and Mari Lowe Center for Comparative Oncology, University of Pennsylvania School of Veterinary Medicine, Kennett Square, Pennsylvania 19348, USA.

出版信息

Biol Reprod. 2009 Jul;81(1):46-55. doi: 10.1095/biolreprod.108.075390. Epub 2009 Mar 4.

Abstract

The major function of sperm is the delivery of the paternal genome to the metaphase II oocyte, ensuring transmission of the genetic information to the next generation. For successful fertilization and healthy offspring, sperm DNA must be protected from exogenous insults. This is achieved by packaging the sperm DNA into a condensed protamine-bound form, preceded by the precisely orchestrated removal of histones and intermittent insertion and removal of transition proteins. This remodeling process requires relaxation of supercoiled DNA by transient formation of physiological strand breaks that spermatids, being haploid, cannot repair by homologous recombination. In somatic cells, the presence of DNA strand breaks rapidly induces the formation of poly(ADP-ribose) by nuclear poly(ADP-ribose) polymerases, which in turn facilitates DNA strand break signaling and assembly of DNA repair complexes. We reported earlier that chromatin remodeling steps during spermiogenesis trigger poly(ADP-ribose) (PAR) formation. Here, we show that knockout mice deficient in PARP1, PARG (110-kDa isoform), or both display morphological and functional sperm abnormalities that are dependent on the individual genotypes, including residual DNA strand breaks associated with varying degrees of subfertility. The data presented highlight the importance of PAR metabolism, particularly PARG function, as a prerequisite of proper sperm chromatin quality.

摘要

精子的主要功能是将父本基因组传递给中期II卵母细胞,确保遗传信息传递给下一代。为了成功受精并孕育健康后代,精子DNA必须免受外源损伤。这是通过将精子DNA包装成与鱼精蛋白结合的浓缩形式来实现的,在此之前需要精确地有序去除组蛋白,并间歇性地插入和去除过渡蛋白。这种重塑过程需要通过生理链断裂的瞬时形成来松弛超螺旋DNA,而单倍体的精子细胞无法通过同源重组修复这种链断裂。在体细胞中,DNA链断裂的存在会迅速诱导核多聚(ADP-核糖)聚合酶形成多聚(ADP-核糖),进而促进DNA链断裂信号传导和DNA修复复合物的组装。我们之前报道过精子发生过程中的染色质重塑步骤会触发多聚(ADP-核糖)(PAR)的形成。在此,我们表明,缺乏PARP1、PARG(110 kDa异构体)或两者的基因敲除小鼠表现出形态和功能上的精子异常,这些异常取决于个体基因型,包括与不同程度的生育力低下相关的残留DNA链断裂。所呈现的数据突出了PAR代谢,特别是PARG功能作为精子染色质质量正常的先决条件的重要性。

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