| Literature DB >> 34108658 |
Ruibao Su1,2, Li-Hua Fan3,4, Changchang Cao1, Lei Wang1,5, Zongchang Du1,2, Zhaokui Cai1,2, Ying-Chun Ouyang4, Yue Wang2,4, Qian Zhou2,4, Ligang Wu6, Nan Zhang7, Xiaoxiao Zhu1,2, Wen-Long Lei4, Hailian Zhao1,2, Yong Tian1,2, Shunmin He1, Catherine C L Wong8,9,10,11, Qing-Yuan Sun12,13, Yuanchao Xue14,15.
Abstract
RNA-binding proteins (RBPs) have essential functions during germline and early embryo development. However, current methods are unable to identify the in vivo targets of a RBP in these low-abundance cells. Here, by coupling RBP-mediated reverse transcription termination with linear amplification of complementary DNA ends and sequencing, we present the LACE-seq method for identifying RBP-regulated RNA networks at or near the single-oocyte level. We determined the binding sites and regulatory mechanisms for several RBPs, including Argonaute 2 (Ago2), Mili, Ddx4 and Ptbp1, in mature mouse oocytes. Unexpectedly, transcriptomics and proteomics analysis of Ago2-/- oocytes revealed that Ago2 interacts with endogenous small interfering RNAs (endo-siRNAs) to repress mRNA translation globally. Furthermore, the Ago2 and endo-siRNA complexes fine-tune the transcriptome by slicing long terminal repeat retrotransposon-derived chimeric transcripts. The precise mapping of RBP-binding sites in low-input cells opens the door to studying the roles of RBPs in embryonic development and reproductive diseases.Entities:
Year: 2021 PMID: 34108658 DOI: 10.1038/s41556-021-00696-9
Source DB: PubMed Journal: Nat Cell Biol ISSN: 1465-7392 Impact factor: 28.824