Trypanosome mRNA recapping is triggered by hypermethylation originating from cap 4

Author:

Ignatochkina Anna V1,Iguchi Jesavel A1,Kore Anilkumar R2,Ho C Kiong1ORCID

Affiliation:

1. Department of Infection Biology, Graduate School of Comprehensive Human Sciences, Institute of Medicine, University of Tsukuba , Ibaraki 305-8575 , Japan

2. Life Sciences Solutions Group, Thermo Fisher Scientific , 2130 Woodward Street, Austin , TX  78744-1832 , USA

Abstract

Abstract RNA methylation adjacent to the 5′ cap plays a critical role in controlling mRNA stability and protein synthesis. In trypanosomes the 5′-terminus of mRNA is protected by hypermethylated cap 4. Trypanosomes encode a cytoplasmic recapping enzyme TbCe1 which possesses an RNA kinase and guanylyltransferase activities that can convert decapped 5′-monophosphate-terminated pRNA into GpppRNA. Here, we demonstrated that the RNA kinase activity is stimulated by two orders of magnitude on a hypermethylated pRNA derived from cap 4. The N6, N6-2′-O trimethyladenosine modification on the first nucleotide was primarily accountable for enhancing both the RNA kinase and the guanylyltransferase activity of TbCe1. In contrast, N6 methyladenosine severely inhibits the guanylyltransferase activity of the mammalian capping enzyme. Furthermore, we showed that TbCmt1 cap (guanine N7) methyltransferase was localized in the cytoplasm, and its activity was also stimulated by hypermethylation at 2′-O ribose, suggesting that TbCe1 and TbCmt1 act together as a recapping enzyme to regenerate translatable mRNA from decapped mRNA. Our result establishes the functional role of cap 4 hypermethylation in recruitment and activation of mRNA recapping pathway. Methylation status at the 5′-end of transcripts could serve as a chemical landmark to selectively regulate the level of functional mRNA by recapping enzymes.

Funder

KAKENHI

University of Tsukuba

Publisher

Oxford University Press (OUP)

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