Human RNase 4 improves mRNA sequence characterization by LC–MS/MS

Author:

Wolf Eric J1,Grünberg Sebastian1,Dai Nan1,Chen Tien-Hao1,Roy Bijoyita1ORCID,Yigit Erbay1ORCID,Corrêa Ivan R1ORCID

Affiliation:

1. New England Biolabs, Inc , 43/44 Dunham Ridge, Beverly, MA 01915, USA

Abstract

Abstract With the rapid growth of synthetic messenger RNA (mRNA)-based therapeutics and vaccines, the development of analytical tools for characterization of long, complex RNAs has become essential. Tandem liquid chromatography–mass spectrometry (LC–MS/MS) permits direct assessment of the mRNA primary sequence and modifications thereof without conversion to cDNA or amplification. It relies upon digestion of mRNA with site-specific endoribonucleases to generate pools of short oligonucleotides that are then amenable to MS-based sequence analysis. Here, we showed that the uridine-specific human endoribonuclease hRNase 4 improves mRNA sequence coverage, in comparison with the benchmark enzyme RNase T1, by producing a larger population of uniquely mappable cleavage products. We deployed hRNase 4 to characterize mRNAs fully substituted with 1-methylpseudouridine (m1Ψ) or 5-methoxyuridine (mo5U), as well as mRNAs selectively depleted of uridine–two key strategies to reduce synthetic mRNA immunogenicity. Lastly, we demonstrated that hRNase 4 enables direct assessment of the 5′ cap incorporation into in vitro transcribed mRNA. Collectively, this study highlights the power of hRNase 4 to interrogate mRNA sequence, identity, and modifications by LC–MS/MS.

Funder

New England Biolabs

Publisher

Oxford University Press (OUP)

Subject

Genetics

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