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组蛋白去乙酰化酶抑制可改善克隆小鼠胚胎核糖体 RNA 基因的激活和胚胎核仁重编程。

Histone deacetylase inhibition improves activation of ribosomal RNA genes and embryonic nucleolar reprogramming in cloned mouse embryos.

机构信息

Department of Animal Biotechnology, College of Animal Bioscience and Biotechnology/Animal Resources Research Center, Konkuk University, Seoul, Republic of Korea.

出版信息

Biol Reprod. 2011 Nov;85(5):1048-56. doi: 10.1095/biolreprod.110.089474. Epub 2011 Jul 13.

Abstract

Our group found that the treatment of embryos with histone deacetylase inhibitors (HDACi), including trichostatin A, Scriptaid, suberoylanilide hydroxamic acid, and oxamflatin, after cloning by somatic cell nuclear transfer (SCNT) resulted in significantly improved efficiency. Although many researchers have investigated the use of HDACi treatment to improve the quality of cloned mouse embryos, the mechanism underlying this treatment has not been completely understood. We believe that the effect of HDACi on embryonic gene activation (EGA) is important for normal development of cloned embryos. In the present study, using highly sensitive fluorescence in situ hybridization (FISH) with probes complementary to mouse rDNA, the effect of Scriptaid on the onset of rRNA synthesis was examined in cloned embryos. In addition, to determine how Scriptaid affects pre-rRNA processing machinery in SCNT embryos with activated rDNA transcription, functional nucleolar formation was analyzed in detail by combined assessment of rRNA synthesis and nucleolar protein allocation in preimplantation embryos. In this experiment, at least part of the rRNA localization by FISH was substituted by 5-bromouridine 5'-triphosphate staining after alpha-amanitin treatment. The results show that in the late 2-cell stage, a number of SCNT embryos initiated transcriptional activation while having one blastomere showing inactivated rRNA transcription and another blastomere showing activated rRNA transcription and despite both nuclei being in interphase. In addition, in some SCNT embryos, the same nuclei contained a mixture of inactively and actively transcribed rRNA, which was rarely observed in intracytoplasmic sperm injection embryos. This asynchronous transcription induced a delay of one cell cycle in SCNT embryo activation of functional nucleoli. Scriptaid can overcome this failure in the timely onset of embryonic gene transcription by activation of rRNA genes and promotion of nucleolar protein allocation during the early phase of EGA.

摘要

我们的研究小组发现,在体细胞核移植(SCNT)后,用组蛋白去乙酰化酶抑制剂(HDACi)处理胚胎,包括曲古抑菌素 A、Scriptaid、丁酸钠和 oxamflatin,可以显著提高效率。尽管许多研究人员已经研究了使用 HDACi 处理来改善克隆小鼠胚胎的质量,但这种处理的机制尚未完全理解。我们认为,HDACi 对胚胎基因激活(EGA)的影响对于克隆胚胎的正常发育很重要。在本研究中,我们使用高度敏感的荧光原位杂交(FISH)技术,用与小鼠 rDNA 互补的探针,研究了 Scriptaid 对克隆胚胎 rRNA 合成起始的影响。此外,为了确定 Scriptaid 如何影响激活 rDNA 转录的 SCNT 胚胎中的前 rRNA 加工机制,我们通过在植入前胚胎中综合评估 rRNA 合成和核仁蛋白分配,详细分析了功能核仁的形成。在这个实验中,在用 alpha-amanitin 处理后,至少一部分 FISH 定位的 rRNA 被 5-溴尿嘧啶 5'-三磷酸染色取代。结果表明,在晚期 2 细胞阶段,许多 SCNT 胚胎启动转录激活,同时一个卵裂球显示 rRNA 转录失活,另一个卵裂球显示 rRNA 转录激活,尽管两个核都处于间期。此外,在一些 SCNT 胚胎中,同一核内含有混合的失活和活跃转录的 rRNA,这在胞质内精子注射胚胎中很少观察到。这种异步转录导致 SCNT 胚胎的功能核仁激活延迟一个细胞周期。Scriptaid 可以通过激活 rRNA 基因和促进核仁蛋白在 EGA 的早期分配来克服胚胎基因转录的这种启动延迟。

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