首页> 外文期刊>Genes and Development: a Journal Devoted to the Molecular Analysis of Gene Expression in Eukaryotes, Prokaryotes, and Viruses >Rapid embryonic cell cycles defer the establishment of heterochromatin by Eggless/SetDB1 in Drosophila
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Rapid embryonic cell cycles defer the establishment of heterochromatin by Eggless/SetDB1 in Drosophila

机译:快速的胚胎细胞循环通过果蝇的蛋白/ setdb1推迟建立异料蛋白

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摘要

Acquisition of chromatin modifications during embryogenesis distinguishes different regions of an initially naive genome. In many organisms, repetitive DNA is packaged into constitutive heterochromatin that is marked by di/trimethylation of histone H3K9 and the associated protein HP1a. These modifications enforce the unique epigenetic properties of heterochromatin. However, in the early Drosophila melanogaster embryo, the heterochromatin lacks these modifications, which appear only later, when rapid embryonic cell cycles slow down at the midblastula transition (MBT). Here we focus on the initial steps restoring heterochromatic modifications in the embryo. We describe the JabbaTrap, a technique for inactivating maternally provided proteins in embryos. Using the JabbaTrap, we reveal a major requirement for the methyltransferase Eggless/SetDB1 in the establishment of heterochromatin. In contrast, other methyltransf erases contribute minimally. Live imaging reveals that endogenous Eggless gradually accumulates on chromatin in interphase but then dissociates in mitosis, and its accumulation must restart in the next cell cycle. Cell cycle slowing as the embryo approaches the MBT permits increasing accumulation and action of Eggless at its targets. Experimental manipulation of interphase duration shows that cell cycle speed regulates Eggless. We propose that developmental slowing of the cell cycle times embryonic heterochromatin formation.
机译:在胚胎发生过程中获取染色质修饰区分初始Naive基因组的不同区域。在许多生物中,重复的DNA被包装成组成型异铬胺,其由组蛋白H3K9的二甲基化和相关蛋白质HP1A标记。这些修饰强制了异铬胺的独特表观遗传性质。然而,在早期的果蝇黑素转酯胚胎中,异铬胺缺乏这些修饰,其仅在后来出现,当时胚胎细胞循环在中间玻璃孢菌过渡(MBT)上慢下来。在这里,我们专注于恢复胚胎中的初始步骤。我们描述了Jabbatrap,一种用于在胚胎中灭活母体蛋白质的技术。使用Jabbatrap,我们揭示了甲基转移酶蛋白/ SetdB1在建立异铬胺中的主要要求。相比之下,其他甲基转移擦除源于微小的贡献。实时成像显示内源性蛋黄在间间逐渐积聚在染色质上,然后在有丝分裂中解离,并且其积聚必须在下一个细胞周期中重启。随着胚胎接近胚胎在其目标上允许增加蛋蛋的累积和动作,细胞周期减速。双相持续时间的实验操纵表明,细胞周期速度调节蛋。我们提出了细胞循环时间胚胎异铬胺蛋白形成的发育减慢。

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