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Programmable RNA N6-methyladenosine editing by CRISPR-Cas9 conjugates.


ABSTRACT: RNA modification in the form of N6-methyladenosine (m6A) regulates nearly all the post-transcriptional processes. The asymmetric m6A deposition suggests that regional methylation may have distinct functional consequences. However, current RNA biology tools do not distinguish the contribution of individual m6A modifications. Here we report the development of 'm6A editing', a powerful approach that enables m6A installation and erasure from cellular RNAs without changing the primary sequence. We engineered fusions of CRISPR-Cas9 and a single-chain m6A methyltransferase that can be programmed with a guide RNA. The resultant m6A 'writers' allow functional comparison of single site methylation in different messenger RNA regions. We further engineered m6A 'erasers' by fusing CRISPR-Cas9 with ALKBH5 or FTO to achieve site-specific demethylation of RNAs. The development of programmable m6A editing not only expands the scope of RNA engineering, but also facilitates mechanistic understanding of epitranscriptome.

SUBMITTER: Liu XM 

PROVIDER: S-EPMC6702037 | biostudies-literature | 2019 Sep

REPOSITORIES: biostudies-literature

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Programmable RNA N<sup>6</sup>-methyladenosine editing by CRISPR-Cas9 conjugates.

Liu Xiao-Min XM   Zhou Jun J   Mao Yuanhui Y   Ji Quanquan Q   Qian Shu-Bing SB  

Nature chemical biology 20190805 9


RNA modification in the form of N<sup>6</sup>-methyladenosine (m<sup>6</sup>A) regulates nearly all the post-transcriptional processes. The asymmetric m<sup>6</sup>A deposition suggests that regional methylation may have distinct functional consequences. However, current RNA biology tools do not distinguish the contribution of individual m<sup>6</sup>A modifications. Here we report the development of 'm<sup>6</sup>A editing', a powerful approach that enables m<sup>6</sup>A installation and erasu  ...[more]

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