2’,3’‐Protected Nucleotides as Building Blocks for Enzymatic de novo RNA Synthesis

Author:

Pichon Maëva1ORCID,Levi‐Acobas Fabienne1,Kitoun Camélia1,Hollenstein Marcel1ORCID

Affiliation:

1. Institut Pasteur Université Paris Cité CNRS UMR3523 Department of Structural Biology and Chemistry Laboratory for Bioorganic Chemistry of Nucleic Acids 28, rue du Docteur Roux, 75724 Paris Cedex 15 France

Abstract

AbstractBesides being a key player in numerous fundamental biological processes, RNA also represents a versatile platform for the creation of therapeutic agents and efficient vaccines. The production of RNA oligonucleotides, especially those decorated with chemical modifications, cannot meet the exponential demand. Due to the inherent limits of solid‐phase synthesis and in vitro transcription, alternative, biocatalytic approaches are in dire need to facilitate the production of RNA oligonucleotides. Here, we present a first step towards the controlled enzymatic synthesis of RNA oligonucleotides. We have explored the possibility of a simple protection step of the vicinal cis‐diol moiety to temporarily block ribonucleotides. We demonstrate that pyrimidine nucleotides protected with acetals, particularly 2′,3′‐O‐isopropylidene, are well‐tolerated by the template‐independent RNA polymerase PUP (polyU polymerase) and highly efficient coupling reactions can be achieved within minutes – an important feature for the development of enzymatic de novo synthesis protocols. Even though purines are not equally well‐tolerated, these findings clearly demonstrate the possibility of using cis‐diol‐protected ribonucleotides combined with template‐independent polymerases for the stepwise construction of RNA oligonucleotides.

Funder

Institut Pasteur

Sanofi

Publisher

Wiley

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