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5´XP sRNA-seq:高效鉴定具有和不具有 5´磷酸化的转录本,揭示进化保守的小 RNA。

5´XP sRNA-seq: efficient identification of transcripts with and without 5´ phosphorylation reveals evolutionary conserved small RNA.

机构信息

Department of Biomedical and Clinical Sciences, Linköping University, Linköping, Sweden.

Department of Microbiology, Tumor and Cell Biology, Science for Life Laboratory, Karolinska Institute, Stockholm.

出版信息

RNA Biol. 2021 Nov;18(11):1588-1599. doi: 10.1080/15476286.2020.1861770. Epub 2020 Dec 31.

Abstract

Small RNA (sRNA) sequencing has been critical for our understanding of many cellular processes, including gene regulation. Nonetheless, the varying biochemical properties of sRNA, such as 5´ nucleotide modifications, make many sRNA subspecies incompatible with common protocols for sRNA sequencing. Here we describe 5XP-seq that outlines a novel strategy that captures a more complete picture of sRNA. By tagging 5´P sRNA during library preparation, 5XP-seq combines an open approach that includes all types of 5'-terminal modifications (5´X), with a selective approach for 5-phosphorylated sRNA (5´P). We show that 5XP-seq not only enriches phosphorylated miRNA and piRNA but successfully discriminates these sRNA from all other sRNA species. We further demonstrate the importance of this strategy by successful inter-species validation of sRNAs that would have otherwise failed, including human to insect translation of several tRNA (tRFs) and rRNA (rRFs) fragments. By combining 5´ insensitive library strategies with 5´ sensitive tagging, we have successfully tackled an intrinsic bias in modern sRNA sequencing that will help us reveal the true complexity and the evolutionary significance of the sRNA world.

摘要

小 RNA (sRNA) 测序对于我们理解许多细胞过程至关重要,包括基因调控。尽管如此,sRNA 的各种生化特性,如 5´核苷酸修饰,使得许多 sRNA 亚种与 sRNA 测序的常见方案不兼容。在这里,我们描述了 5XP-seq,它概述了一种新的策略,可以更全面地描绘 sRNA。通过在文库制备过程中标记 5´P sRNA,5XP-seq 结合了一种开放的方法,包括所有类型的 5´-末端修饰(5´X),以及针对 5´-磷酸化 sRNA(5´P)的选择性方法。我们表明,5XP-seq 不仅可以富集磷酸化的 miRNA 和 piRNA,而且可以成功区分这些 sRNA 与所有其他 sRNA 种类。我们通过成功地验证了本来会失败的跨物种 sRNA,进一步证明了这种策略的重要性,包括几个人类到昆虫的 tRNA (tRFs) 和 rRNA (rRFs) 片段的翻译。通过将 5´不敏感文库策略与 5´敏感标记相结合,我们成功地解决了现代 sRNA 测序中的固有偏差,这将帮助我们揭示 sRNA 世界的真正复杂性和进化意义。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/441e/8594926/0ffc374887e1/KRNB_A_1861770_F0001_C.jpg

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