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西亚试剂:Piwi蛋白在转位子沉默中的作用

 

The endonuclease activity of Mili fuels piRNA amplification that silences LINE1 elements。

Serena De Fazio, Nenad Bartonicek, Monica Di Giacomo, Cei Abreu-Goodger, Aditya Sankar, Charlotta Funaya, Claude Antony, Pedro N. Moreira, Anton J. Enright & Dónal O’Carroll

 

Piwi proteins and Piwi-interacting RNAs (piRNAs) have conserved functions in transposon silencing1. The murine Piwi proteins Mili and Miwi2 (also called Piwil2 and Piwil4, respectively) direct epigenetic LINE1 and intracisternal A particle transposon silencing during genome reprogramming in the embryonic male germ line2, 3, 4. Piwi proteins are proposed to be piRNA-guided endonucleases that initiate secondary piRNA biogenesis5, 6, 7; however, the actual contribution of their endonuclease activities to piRNA biogenesis and transposon silencing remain unknown. To investigate the role of Piwi-catalysed endonucleolytic activity, we engineered point mutations in mice that substitute the second aspartic acid to an alanine in the DDH catalytic triad of Mili and Miwi2, generating the MiliDAH and Miwi2DAH alleles, respectively. Analysis of Mili-bound piRNAs from homozygous MiliDAH fetal gonadocytes revealed a failure of transposon piRNA amplification, resulting in the marked reduction of piRNA bound within Miwi2 ribonuclear particles. We find that Mili-mediated piRNA amplification is selectively required for LINE1, but not intracisternal A particle, silencing. The defective piRNA pathway in MiliDAH mice results in spermatogenic failure and sterility. Surprisingly, homozygous Miwi2DAH mice are fertile, transposon silencing is established normally and no defects in secondary piRNA biogenesis are observed. In addition, the hallmarks of piRNA amplification are observed in Miwi2-deficient gonadocytes. We conclude that cycles of intra-Mili secondary piRNA biogenesis fuel piRNA amplification that is absolutely required for LINE1 silencing..

近日,国际著名杂志Nature刊登了意大利研究者的最新研究成果“The endonuclease activity of Mili fuels piRNA amplification that silences LINE1 elements。”

Piwi蛋白与同它们相关的“Piwi相互作用RNA”(piRNA)的组合,调控动物生殖细胞系中的“外成转位子沉默作用”。Piwi蛋白被预测是核酸内切酶,但这种活性的重要性过去却未在活体中演示过。现在,Dónal O\'Carroll 和 Ramesh Pillai的实验室已培育出了小鼠模型,在其中,预计对在小鼠的三个Piwi蛋白Mili、Miwi 和 Miwi2中的核酸酶活性至关重要的残体都发生了突变。突变的小鼠表现出表现型差异。Mili 和 Miwi突变体在piRNA生成、转位子沉默作用和繁殖力方面是有缺陷的,而Miwi2突变体则有正常的piRNA水平,似乎在进行piRNA放大,并且使转位子沉默。这些研究突显了负责piRNA生物生成的鼠科动物的各种酶之间的差别