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本文引用的文献

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Chromatin signature reveals over a thousand highly conserved large non-coding RNAs in mammals.染色质特征揭示了哺乳动物中一千多种高度保守的大型非编码RNA。
Nature. 2009 Mar 12;458(7235):223-7. doi: 10.1038/nature07672. Epub 2009 Feb 1.
2
Genome-wide profiling of salt fractions maps physical properties of chromatin.盐组分的全基因组分析描绘了染色质的物理特性。
Genome Res. 2009 Mar;19(3):460-9. doi: 10.1101/gr.087619.108. Epub 2008 Dec 16.
3
CTCFL/BORIS is a methylation-independent DNA-binding protein that preferentially binds to the paternal H19 differentially methylated region.CTCFL/BORIS是一种不依赖甲基化的DNA结合蛋白,它优先结合父本H19差异甲基化区域。
Cancer Res. 2008 Jul 15;68(14):5546-51. doi: 10.1158/0008-5472.CAN-08-1005.
4
Maternal depletion of CTCF reveals multiple functions during oocyte and preimplantation embryo development.母源CTCF缺失揭示了其在卵母细胞和植入前胚胎发育过程中的多种功能。
Development. 2008 Aug;135(16):2729-38. doi: 10.1242/dev.024539. Epub 2008 Jul 9.
5
Integration of external signaling pathways with the core transcriptional network in embryonic stem cells.胚胎干细胞中外部信号通路与核心转录网络的整合。
Cell. 2008 Jun 13;133(6):1106-17. doi: 10.1016/j.cell.2008.04.043.
6
Characterization of nucleohistone and nucleoprotamine components in the mature human sperm nucleus.成熟人类精子细胞核中核组蛋白和核精蛋白成分的表征
Asian J Androl. 2008 Jul;10(4):535-41. doi: 10.1111/j.1745-7262.2008.00410.x.
7
Sperm-derived histones contribute to zygotic chromatin in humans.精子来源的组蛋白对人类合子染色质有贡献。
BMC Dev Biol. 2008 Mar 31;8:34. doi: 10.1186/1471-213X-8-34.
8
Widespread epigenetic abnormalities suggest a broad DNA methylation erasure defect in abnormal human sperm.广泛的表观遗传异常表明异常人类精子中存在广泛的DNA甲基化消除缺陷。
PLoS One. 2007 Dec 12;2(12):e1289. doi: 10.1371/journal.pone.0001289.
9
Differences between homologous alleles of olfactory receptor genes require the Polycomb Group protein Eed.嗅觉受体基因同源等位基因之间的差异需要多梳蛋白家族蛋白Eed。
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Genome-wide maps of chromatin state in pluripotent and lineage-committed cells.多能细胞和谱系定向细胞中染色质状态的全基因组图谱。
Nature. 2007 Aug 2;448(7153):553-60. doi: 10.1038/nature06008. Epub 2007 Jul 1.

人类精子染色质的核酸内切酶敏感区域在启动子和CTCF结合序列中高度富集。

Endonuclease-sensitive regions of human spermatozoal chromatin are highly enriched in promoter and CTCF binding sequences.

作者信息

Arpanahi Ali, Brinkworth Martin, Iles David, Krawetz Stephen A, Paradowska Agnieszka, Platts Adrian E, Saida Myriam, Steger Klaus, Tedder Philip, Miller David

机构信息

Reproduction and Early Development Unit, Leeds Institute of Genetics and Health Therapeutics, University of Leeds, Leeds, United Kingdom.

出版信息

Genome Res. 2009 Aug;19(8):1338-49. doi: 10.1101/gr.094953.109. Epub 2009 Jul 7.

DOI:10.1101/gr.094953.109
PMID:19584098
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2720182/
Abstract

During the haploid phase of mammalian spermatogenesis, nucleosomal chromatin is ultimately repackaged by small, highly basic protamines to generate an extremely compact, toroidal chromatin architecture that is critical to normal spermatozoal function. In common with several species, however, the human spermatozoon retains a small proportion of its chromatin packaged in nucleosomes. As nucleosomal chromatin in spermatozoa is structurally more open than protamine-packaged chromatin, we considered it likely to be more accessible to exogenously applied endonucleases. Accordingly, we have used this premise to identify a population of endonuclease-sensitive DNA sequences in human and murine spermatozoa. Our results show unequivocally that, in contrast to the endonuclease-resistant sperm chromatin packaged by protamines, regions of increased endonuclease sensitivity are closely associated with gene regulatory regions, including many promoter sequences and sequences recognized by CCCTC-binding factor (CTCF). Similar differential packaging of promoters is observed in the spermatozoal chromatin of both mouse and man. These observations imply the existence of epigenetic marks that distinguish gene regulatory regions in male germ cells and prevent their repackaging by protamines during spermiogenesis. The ontology of genes under the control of endonuclease-sensitive regulatory regions implies a role for this phenomenon in subsequent embryonic development.

摘要

在哺乳动物精子发生的单倍体阶段,核小体染色质最终被小的、高度碱性的鱼精蛋白重新包装,以形成一种极其紧凑的环形染色质结构,这对正常精子功能至关重要。然而,与几个物种一样,人类精子保留了一小部分包装在核小体中的染色质。由于精子中的核小体染色质在结构上比鱼精蛋白包装的染色质更开放,我们认为它可能更容易被外源应用核酸内切酶接近。因此,我们利用这一前提在人类和小鼠精子中鉴定出一群对核酸内切酶敏感的DNA序列。我们的结果明确表明,与由鱼精蛋白包装的对核酸内切酶有抗性的精子染色质相反,核酸内切酶敏感性增加的区域与基因调控区域密切相关,包括许多启动子序列和被CCCTC结合因子(CTCF)识别的序列。在小鼠和人类的精子染色质中都观察到了类似的启动子差异包装。这些观察结果意味着存在表观遗传标记,这些标记区分雄性生殖细胞中的基因调控区域,并在精子发生过程中防止它们被鱼精蛋白重新包装。受核酸内切酶敏感调控区域控制的基因的本体论意味着这种现象在随后的胚胎发育中起作用。