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敏化 piRNA 报告基因鉴定出多个 RNA 加工因子参与 piRNA 介导的基因沉默。

Sensitized piRNA reporter identifies multiple RNA processing factors involved in piRNA-mediated gene silencing.

机构信息

Department of Molecular Genetics and Cell Biology, University of Chicago, Chicago, IL 60637, USA.

Department of Laboratory Medicine, Third Affiliated Hospital of Sun Yat-Sen University, Guangzhou, Guangdong Province 510000, China.

出版信息

Genetics. 2023 Aug 9;224(4). doi: 10.1093/genetics/iyad095.

Abstract

Metazoans guard their germlines against transposons and other foreign transcripts with PIWI-interacting RNAs (piRNAs). Due to the robust heritability of the silencing initiated by piRNAs in Caenorhabditis elegans (C. elegans), previous screens using C. elegans were strongly biased to uncover members of this pathway in the maintenance process but not in the initiation process. To identify novel piRNA pathway members, we have utilized a sensitized reporter strain which detects defects in initiation, amplification, or regulation of piRNA silencing. Using our reporter, we have identified Integrator complex subunits, nuclear pore components, protein import components, and pre-mRNA splicing factors as essential for piRNA-mediated gene silencing. We found the small nuclear processing cellular machine termed the Integrator complex is required for both type I and type II piRNA production. Notably, we identified a role for nuclear pore and nucleolar components NPP-1/Nup54, NPP-6/Nup160, NPP-7/Nup153, and FIB-1 in promoting the perinuclear localization of anti-silencing CSR-1 Argonaute, as well as a role for Importin factor IMA-3 in nuclear localization of silencing Argonaute HRDE-1. Together, we have shown that piRNA silencing in C. elegans is dependent on evolutionarily ancient RNA processing machinery that has been co-opted to function in the piRNA-mediated genome surveillance pathway.

摘要

后生动物通过 PIWI 相互作用 RNA(piRNA)来保护其生殖细胞免受转座子和其他外来转录本的侵害。由于在秀丽隐杆线虫(C. elegans)中由 piRNA 引发的沉默具有很强的遗传性,因此之前使用 C. elegans 进行的筛选强烈偏向于在维持过程中而不是在起始过程中发现该途径的成员。为了鉴定新的 piRNA 途径成员,我们利用了一种敏感的报告菌株,该菌株可检测到 piRNA 沉默的起始、扩增或调节中的缺陷。使用我们的报告,我们鉴定了整合体复合物亚基、核孔成分、蛋白导入成分和 pre-mRNA 剪接因子是 piRNA 介导的基因沉默所必需的。我们发现,被称为整合体复合物的小型核处理细胞机器对于 I 型和 II 型 piRNA 的产生都是必需的。值得注意的是,我们确定了核孔和核仁成分 NPP-1/Nup54、NPP-6/Nup160、NPP-7/Nup153 和 FIB-1 在促进抗沉默 CSR-1 Argonaute 的核周定位中的作用,以及 Importin 因子 IMA-3 在沉默 Argonaute HRDE-1 的核定位中的作用。总之,我们表明,C. elegans 中的 piRNA 沉默依赖于进化上古老的 RNA 处理机制,该机制已被篡夺用于 piRNA 介导的基因组监测途径。

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