Profiling of circular RNA N6‐methyladenosine in moso bamboo (Phyllostachys edulis) using nanopore‐based direct RNA sequencing

Autor:	Ximei Han, Hangxiao Zhang, Lianfeng Gu, Huihui Wang, Qianyue Zhang, Yongsheng Wang, Yushan Zheng, Qiang Zhu, Feihu Xi, Anireddy S. N. Reddy, Markus V. Kohnen, Huiyuan Wang, Wentao Wei
Rok vydání:	2020
Předmět:	RNA metabolism biology Chemistry RNA Plant Science Computational biology biology.organism_classification Biochemistry General Biochemistry Genetics and Molecular Biology Nanopore chemistry.chemical_compound Phyllostachys edulis Circular RNA splice Exact location N6-Methyladenosine
Zdroj:	Journal of Integrative Plant Biology. 62:1823-1838
ISSN:	1744-7909 1672-9072
Popis:	N6 -methyladenosine (m6 A) is a prevalent modification in messenger RNAs and circular RNAs that play important roles in regulating various aspects of RNA metabolism. However, the occurrence of the m6 A modification in plant circular RNAs has not been reported. A widely used method to identify m6 A modifications relies on m6 A-specific antibodies followed by next-generation sequencing of precipitated RNAs (MeRIP-Seq). However, one limitation of MeRIP-Seq is that it does not provide the precise location of m6 A at single-nucleotide resolution. Although more recent sequencing techniques such as Nanopore-based direct RNA sequencing (DRS) can overcome such limitations, the technology does not allow sequencing of circular RNAs, as these molecules lack a poly(A) tail. Here, we developed a novel method to detect the precise location of m6 A modifications in circular RNAs using Nanopore DRS. We first enriched our samples for circular RNAs, which we then fragmented and sequenced on the Nanopore platform with a customized protocol. Using this method, we identified 470 unique circular RNAs from DRS reads based on the back-spliced junction region. Among exonic circular RNAs, about 10% contained m6 A sites, which mainly occurred around acceptor and donor splice sites. This study demonstrates the utility of our antibody-independent method in identifying total and methylated circular RNAs using Nanopore DRS. This method has the additional advantage of providing the exact location of m6 A sites at single-base resolution in circular RNAs or linear transcripts from non-coding RNA without poly(A) tails.
Databáze:	OpenAIRE
Externí odkaz:	https://explore.openaire.eu/search/publication?articleId=doi_________::e9184233d2c9f0cf1c390061c031a73b https://doi.org/10.1111/jipb.13002 Zobrazit plný text záznamu Plný text ve formátu PDF Plný text ve formátu HTML
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