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PRMT1 甲基化刚地弓形虫的单个 Argonaute,并对于招募 Tudor 核酸内切酶用于反义向导 RNA 对靶 RNA 的切割很重要。

PRMT1 methylates the single Argonaute of Toxoplasma gondii and is important for the recruitment of Tudor nuclease for target RNA cleavage by antisense guide RNA.

机构信息

Department of Biochemistry and Molecular Biology, University of South Alabama, College of Medicine, 307 University Blvd., Mobile, Alabama, USA.

出版信息

Cell Microbiol. 2012 Jun;14(6):882-901. doi: 10.1111/j.1462-5822.2012.01763.x. Epub 2012 Feb 28.

DOI:10.1111/j.1462-5822.2012.01763.x
PMID:22309152
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3682492/
Abstract

Argonaute (Ago) plays a central role in RNA interference in metazoans, but its status in lower organisms remains ill-defined. We report on the Ago complex of the unicellular protozoan, Toxoplasma gondii (Tg), an obligatory pathogen of mammalian hosts. The PIWI-like domain of TgAgo lacked the canonical DDE/H catalytic triad, explaining its weak target RNA cleavage activity. However, TgAgo associated with a stronger RNA slicer, a Tudor staphylococcal nuclease (TSN), and with a protein Arg methyl transferase, PRMT1. Mutational analysis suggested that the N-terminal RGG-repeat domain of TgAgo was methylated by PRMT1, correlating with the recruitment of TSN. The slicer activity of TgAgo was Mg(2+)-dependent and required perfect complementarity between the guide RNA and the target. In contrast, the TSN activity was Ca(2+) -dependent and required an imperfectly paired guide RNA. Ago knockout parasites showed essentially normal growth, but in contrast, the PRMT1 knockouts grew abnormally. Chemical inhibition of Arg-methylation also had an anti-parasitic effect. These results suggest that the parasitic PRMT1 plays multiple roles, and its loss affects the recruitment of a more potent second slicer to the parasitic RNA silencing complex, the exact mechanism of which remains to be determined.

摘要

Argonaute (Ago) 在后生动物的 RNA 干扰中发挥着核心作用,但它在低等生物中的地位仍未得到明确界定。我们报告了单细胞原生动物刚地弓形虫 (Tg) 的 Ago 复合物,它是哺乳动物宿主的必需病原体。TgAgo 的 PIWI 样结构域缺乏典型的 DDE/H 催化三联体,解释了其较弱的靶 RNA 切割活性。然而,TgAgo 与一种更强的 RNA 切割酶、一个葡萄球菌核酸酶 (TSN) 和一个蛋白质精氨酸甲基转移酶 PRMT1 相关。突变分析表明,TgAgo 的 N 端 RGG 重复结构域被 PRMT1 甲基化,这与 TSN 的募集有关。TgAgo 的切割酶活性依赖于 Mg2+,并且需要向导 RNA 与靶标之间的完全互补。相比之下,TSN 的活性依赖于 Ca2+,并且需要向导 RNA 不完全配对。Ago 敲除寄生虫的生长基本正常,但相反,PRMT1 敲除寄生虫的生长异常。精氨酸甲基化的化学抑制也具有抗寄生虫作用。这些结果表明,寄生的 PRMT1 发挥多种作用,其缺失会影响更有效的第二种切割酶招募到寄生的 RNA 沉默复合物,其确切机制仍有待确定。

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