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LIA5 对于四膜虫大核分化过程中发生的核重排和程序性 DNA 重排是必需的。

LIA5 is required for nuclear reorganization and programmed DNA rearrangements occurring during tetrahymena macronuclear differentiation.

机构信息

Biology Department, Washington University in St. Louis, St. Louis, Missouri, United States of America.

出版信息

PLoS One. 2013 Sep 17;8(9):e75337. doi: 10.1371/journal.pone.0075337. eCollection 2013.

Abstract

During macronuclear differentiation of the ciliate Tetrahymena thermophila, genome-wide DNA rearrangements eliminate nearly 50 Mbp of germline derived DNA, creating a streamlined somatic genome. The transposon-like and other repetitive sequences to be eliminated are identified using a piRNA pathway and packaged as heterochromatin prior to their removal. In this study, we show that LIA5, which encodes a zinc-finger protein likely of transposon origin, is required for both chromosome fragmentation and DNA elimination events. Lia5p acts after the establishment of RNAi-directed heterochromatin modifications, but prior to the excision of the modified sequences. In ∆LIA5 cells, DNA elimination foci, large nuclear sub-structures containing the sequences to be eliminated and the essential chromodomain protein Pdd1p, do not form. Lia5p, unlike Pdd1p, is not stably associated with these structures, but is required for their formation. In the absence of Lia5p, we could recover foci formation by ectopically inducing DNA damage by UV treatment. Foci in both wild-type or UV-treated ∆LIA5 cells contain dephosphorylated Pdd1p. These studies of LIA5 reveal that DNA elimination foci form after the excision of germ-line limited sequences occurs and indicate that Pdd1p reorganization is likely mediated through a DNA damage response.

摘要

在纤毛虫四膜虫的巨核分化过程中,全基因组的 DNA 重排消除了近 50 Mbp 的种系衍生 DNA,从而产生了一个精简的体基因组。通过 piRNA 途径识别要消除的转座子样和其他重复序列,并在去除之前将其包装为异染色质。在这项研究中,我们表明,编码可能起源于转座子的锌指蛋白的 LIA5 对于染色体碎片化和 DNA 消除事件都是必需的。Lia5p 在 RNAi 指导的异染色质修饰建立之后但在修饰序列的切除之前起作用。在 ∆LIA5 细胞中,不形成 DNA 消除焦点、包含要消除的序列的大型核亚结构以及必需的染色质域蛋白 Pdd1p。与 Pdd1p 不同,Lia5p 不会与这些结构稳定相关,但需要它们的形成。在没有 Lia5p 的情况下,我们可以通过 UV 处理异位诱导 DNA 损伤来恢复焦点形成。野生型或经 UV 处理的 ∆LIA5 细胞中的焦点都含有去磷酸化的 Pdd1p。这些对 LIA5 的研究表明,DNA 消除焦点是在种系限制序列切除后形成的,并表明 Pdd1p 的重排可能是通过 DNA 损伤反应介导的。

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